[go: up one dir, main page]
More Web Proxy on the site http://driver.im/

TWI529247B - Anti-human cd52 immunoglobulins - Google Patents

Anti-human cd52 immunoglobulins Download PDF

Info

Publication number
TWI529247B
TWI529247B TW099115371A TW99115371A TWI529247B TW I529247 B TWI529247 B TW I529247B TW 099115371 A TW099115371 A TW 099115371A TW 99115371 A TW99115371 A TW 99115371A TW I529247 B TWI529247 B TW I529247B
Authority
TW
Taiwan
Prior art keywords
seq
antibody
human
light chain
heavy chain
Prior art date
Application number
TW099115371A
Other languages
Chinese (zh)
Other versions
TW201043694A (en
Inventor
布魯斯L 羅伯
史瓦斯 夏卡拉
威廉 哈羅德 布迪克
威廉M 席德斯
Original Assignee
建新公司
Priority date (The priority date is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the date listed.)
Filing date
Publication date
Family has litigation
First worldwide family litigation filed litigation Critical https://patents.darts-ip.com/?family=43085579&utm_source=google_patent&utm_medium=platform_link&utm_campaign=public_patent_search&patent=TWI529247(B) "Global patent litigation dataset” by Darts-ip is licensed under a Creative Commons Attribution 4.0 International License.
Application filed by 建新公司 filed Critical 建新公司
Publication of TW201043694A publication Critical patent/TW201043694A/en
Application granted granted Critical
Publication of TWI529247B publication Critical patent/TWI529247B/en

Links

Classifications

    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K16/00Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies
    • C07K16/18Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies against material from animals or humans
    • C07K16/28Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies against material from animals or humans against receptors, cell surface antigens or cell surface determinants
    • C07K16/2893Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies against material from animals or humans against receptors, cell surface antigens or cell surface determinants against CD52
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K39/00Medicinal preparations containing antigens or antibodies
    • A61K39/395Antibodies; Immunoglobulins; Immune serum, e.g. antilymphocytic serum
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P19/00Drugs for skeletal disorders
    • A61P19/02Drugs for skeletal disorders for joint disorders, e.g. arthritis, arthrosis
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P25/00Drugs for disorders of the nervous system
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P29/00Non-central analgesic, antipyretic or antiinflammatory agents, e.g. antirheumatic agents; Non-steroidal antiinflammatory drugs [NSAID]
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P35/00Antineoplastic agents
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P35/00Antineoplastic agents
    • A61P35/02Antineoplastic agents specific for leukemia
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P37/00Drugs for immunological or allergic disorders
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P37/00Drugs for immunological or allergic disorders
    • A61P37/02Immunomodulators
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P37/00Drugs for immunological or allergic disorders
    • A61P37/02Immunomodulators
    • A61P37/04Immunostimulants
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P37/00Drugs for immunological or allergic disorders
    • A61P37/02Immunomodulators
    • A61P37/06Immunosuppressants, e.g. drugs for graft rejection
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P9/00Drugs for disorders of the cardiovascular system
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N15/00Mutation or genetic engineering; DNA or RNA concerning genetic engineering, vectors, e.g. plasmids, or their isolation, preparation or purification; Use of hosts therefor
    • C12N15/09Recombinant DNA-technology
    • C12N15/63Introduction of foreign genetic material using vectors; Vectors; Use of hosts therefor; Regulation of expression
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K39/00Medicinal preparations containing antigens or antibodies
    • A61K2039/505Medicinal preparations containing antigens or antibodies comprising antibodies
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K2317/00Immunoglobulins specific features
    • C07K2317/20Immunoglobulins specific features characterized by taxonomic origin
    • C07K2317/24Immunoglobulins specific features characterized by taxonomic origin containing regions, domains or residues from different species, e.g. chimeric, humanized or veneered
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K2317/00Immunoglobulins specific features
    • C07K2317/30Immunoglobulins specific features characterized by aspects of specificity or valency
    • C07K2317/34Identification of a linear epitope shorter than 20 amino acid residues or of a conformational epitope defined by amino acid residues
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K2317/00Immunoglobulins specific features
    • C07K2317/50Immunoglobulins specific features characterized by immunoglobulin fragments
    • C07K2317/52Constant or Fc region; Isotype
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K2317/00Immunoglobulins specific features
    • C07K2317/50Immunoglobulins specific features characterized by immunoglobulin fragments
    • C07K2317/56Immunoglobulins specific features characterized by immunoglobulin fragments variable (Fv) region, i.e. VH and/or VL
    • C07K2317/565Complementarity determining region [CDR]
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K2317/00Immunoglobulins specific features
    • C07K2317/60Immunoglobulins specific features characterized by non-natural combinations of immunoglobulin fragments
    • C07K2317/64Immunoglobulins specific features characterized by non-natural combinations of immunoglobulin fragments comprising a combination of variable region and constant region components
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K2317/00Immunoglobulins specific features
    • C07K2317/70Immunoglobulins specific features characterized by effect upon binding to a cell or to an antigen
    • C07K2317/73Inducing cell death, e.g. apoptosis, necrosis or inhibition of cell proliferation
    • C07K2317/732Antibody-dependent cellular cytotoxicity [ADCC]
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K2317/00Immunoglobulins specific features
    • C07K2317/70Immunoglobulins specific features characterized by effect upon binding to a cell or to an antigen
    • C07K2317/73Inducing cell death, e.g. apoptosis, necrosis or inhibition of cell proliferation
    • C07K2317/734Complement-dependent cytotoxicity [CDC]
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K2317/00Immunoglobulins specific features
    • C07K2317/70Immunoglobulins specific features characterized by effect upon binding to a cell or to an antigen
    • C07K2317/76Antagonist effect on antigen, e.g. neutralization or inhibition of binding
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K2317/00Immunoglobulins specific features
    • C07K2317/90Immunoglobulins specific features characterized by (pharmaco)kinetic aspects or by stability of the immunoglobulin
    • C07K2317/94Stability, e.g. half-life, pH, temperature or enzyme-resistance

Landscapes

  • Health & Medical Sciences (AREA)
  • Chemical & Material Sciences (AREA)
  • Organic Chemistry (AREA)
  • Life Sciences & Earth Sciences (AREA)
  • Immunology (AREA)
  • General Health & Medical Sciences (AREA)
  • Medicinal Chemistry (AREA)
  • Engineering & Computer Science (AREA)
  • Bioinformatics & Cheminformatics (AREA)
  • Public Health (AREA)
  • Animal Behavior & Ethology (AREA)
  • Veterinary Medicine (AREA)
  • Pharmacology & Pharmacy (AREA)
  • Nuclear Medicine, Radiotherapy & Molecular Imaging (AREA)
  • General Chemical & Material Sciences (AREA)
  • Chemical Kinetics & Catalysis (AREA)
  • Genetics & Genomics (AREA)
  • Biochemistry (AREA)
  • Biophysics (AREA)
  • Molecular Biology (AREA)
  • Proteomics, Peptides & Aminoacids (AREA)
  • Biomedical Technology (AREA)
  • General Engineering & Computer Science (AREA)
  • Microbiology (AREA)
  • Biotechnology (AREA)
  • Wood Science & Technology (AREA)
  • Zoology (AREA)
  • Rheumatology (AREA)
  • Physics & Mathematics (AREA)
  • Mycology (AREA)
  • Plant Pathology (AREA)
  • Epidemiology (AREA)
  • Heart & Thoracic Surgery (AREA)
  • Orthopedic Medicine & Surgery (AREA)
  • Neurosurgery (AREA)
  • Pain & Pain Management (AREA)
  • Transplantation (AREA)
  • Physical Education & Sports Medicine (AREA)
  • Cardiology (AREA)
  • Neurology (AREA)

Description

抗人CD52免疫球蛋白Anti-human CD52 immunoglobulin

本申請案主張申請於2009年5月13日的美國臨時申請案61/177,837,優先權,該申請案的揭示係以其全文併入做為參考。The present application claims priority to U.S. Provisional Application Serial No. 61/177,837, filed on May 13, 2009, the disclosure of which is hereby incorporated by reference.

本發明係關於一種具有人類CD52(HUCD52)結合專一性的人類化免疫球蛋白。The present invention relates to a humanized immunoglobulin having human CD52 (HUCD52) binding specificity.

CD52為一種在各種正常及惡性淋巴細胞(例如T及B細胞)上大量(500,000分子/細胞)發現的糖基化的糖基磷脂醯肌醇脂質(GPI)-錨定細胞表面蛋白,參考,例如,Hale等.,J Biol regul Homeost Agents 15:386-391(2001);Huh等.,Blood 92: Abstract 4199(1998);Elsner等.,Blood 88:4684-4693(1996);Gilleece等.,Blood 82:807-812(1993);Rodig等.,Clin Cancer Res 12:7174-7179(2006);Ginaldi等.,Leuk Res 22:185-191(1998)。CD52於骨髓樣的細胞有較低的表現量,例如單核細胞、巨噬細胞、及樹突狀細胞,而在成熟自然殺手(NK)細胞、嗜中性球、及多能造血幹細胞有些微表現。Id. CD52亦由附睾及輸精管的上皮細胞產生,及係在通過生殖道期間由精子獲得(Hale等,2001,supra;Domagala等.,Med Sci Monit 7:325-331(2001))。CD52的確切生物功能仍不清楚,但是一些證據顯示其涉及T細胞遷移及共-刺激(Rowan等.,Int Immunol 7:69-77(1995);Masuyama等.,J Exp Med 189:979-989(1999);Watanabe等.,Clin Immunol 120:247-259(2006))。CD52 is a glycosylated phospholipid phosphoinositide lipid (GPI)-anchored cell surface protein found in a large number (500,000 molecules/cell) on various normal and malignant lymphocytes (such as T and B cells), reference, For example, Hale et al., J Biol regul Homeost Agents 15 :386-391 (2001); Huh et al., Blood 92 : Abstract 4199 (1998); Elsner et al., Blood 88 :4684-4693 (1996); Gilleece et al. , Blood 82 : 807-812 (1993); Rodig et al., Clin Cancer Res 12 : 7174-7179 (2006); Ginaldi et al., Leuk Res 22 : 185-191 (1998). CD52 has lower expression in bone marrow-like cells, such as monocytes, macrophages, and dendritic cells, but is slightly different in mature natural killer (NK) cells, neutrophils, and pluripotent hematopoietic stem cells. which performed. Id. CD52 is also produced by epithelial cells of the epididymis and vas deferens, and by sperm during passage through the reproductive tract (Hale et al, 2001, supra ; Domagala et al., Med Sci Monit 7:325-331 (2001)). The exact biological function of CD52 remains unclear, but some evidence suggests that it involves T cell migration and co-stimulation (Rowan et al., Int Immunol 7 : 69-77 (1995); Masuyama et al., J Exp Med 189: 979-989 (1999); Watanabe et al., Clin Immunol 120: 247-259 (2006)).

Campath-(alemtuzumab,,)為一種人類化抗人類CD52單株抗體,其顯現有效力的活體外細胞毒殺效應(ADCC及CDC)。Campath辨識一種抗原決定區,其由成熟CD52蛋白的羧端四個胺基酸及一部份帶負電的GPI錨區所構成。因為其顯著的細胞毒殺效應,Campath能夠活體內消耗CD52陽性細胞及其已證實可用於慢性淋巴性白血病(CLL)的一線及三線治療。已評估Campath用於數種自體免疫疾病的治療,其包含類風濕關節炎、血管炎、肌炎及韋格納氏疾病。然而,Campath的最先進研究在於治療復發型多發性硬化症(MS),這些研究顯示相對於活性比較物(Rebit),其在復發時間有顯著改善。Campath- (alemtuzumab, , ) is a humanized anti-human CD52 monoclonal antibody that exhibits potent in vitro cytotoxic effects (ADCC and CDC). Campath An epitope is identified which consists of the four amino acids at the carboxy terminus of the mature CD52 protein and a portion of the negatively charged GPI anchor region. Because of its significant cytotoxic effect, Campath It is able to consume CD52 positive cells in vivo and its proven first-line and third-line treatment for chronic lymphocytic leukemia (CLL). Campath has been evaluated It is used in the treatment of several autoimmune diseases, including rheumatoid arthritis, vasculitis, myositis and Wegener's disease. However, Campath The most advanced research is in the treatment of relapsing multiple sclerosis (MS), which showed a significant improvement in relapse time relative to the active comparator (Rebit).

仍存在標的CD52的額外醫療劑及方法之需求。There is still a need for additional medical agents and methods for the underlying CD52.

人類化免疫球蛋白Human immunoglobulin

本發明係關於一種具有人類CD52(huCD52)結合專一性的人類化免疫球蛋白,他們可包含老鼠抗人類CD52抗體的互補決定區段(CDRs)。本發明人類化免疫球蛋白具有與其他人類化免疫球蛋白不同,及特別是與包含小鼠抗人類CD52抗體的CDRs的其他人類化免疫球蛋白不同的胺基酸序列。本發明的人類化免疫球蛋白與人類化免疫球蛋白Campath不同。在較佳具體實施例,他們提供比包含Campath的CDRs的人類化抗體更佳的優點。The present invention relates to a humanized immunoglobulin having human CD52 (huCD52) binding specificity, which may comprise complementarity determining segments (CDRs) of mouse anti-human CD52 antibodies. The humanized immunoglobulins of the present invention have amino acid sequences that differ from other humanized immunoglobulins, and in particular, other humanized immunoglobulins comprising CDRs of mouse anti-human CD52 antibodies. Humanized immunoglobulin of the invention and humanized immunoglobulin Campath different. In a preferred embodiment, they provide a ratio that includes Campath The better advantages of humanized antibodies to CDRs.

此處所敘述人類化免疫球蛋白可包含人類化重鏈及人類化輕鏈。在一個具體實施例,人類化免疫球蛋白包含一種含有SEQ ID NO:3的一或更多CDRs(例如,所有三個CDRs)的輕鏈及一種含有SEQ ID NO:16的一或更多CDRs(例如,所有三個CDRs)的重鏈;一種含有SEQ ID NO:4的一或更多CDRs(例如,所有三個CDRs)的輕鏈及一種含有SEQ ID NO:17的一或更多CDRs(例如,所有三個CDRs)的重鏈;一種含有SEQ ID NO:5的一或更多CDRs(例如,所有三個CDRs)的輕鏈及一種含有SEQ ID NO:18的一或更多CDRs(例如,所有三個CDRs)的重鏈;一種含有SEQ ID NO:6的一或更多CDRs(例如,所有三個CDRs)的輕鏈及一種含有SEQ ID NO:19的一或更多CDRs的重鏈;一種含有SEQ ID NO:7的一或更多CDRs(例如,所有三個CDRs)的輕鏈及一種含有SEQ ID NO:20的一或更多CDRs(例如,所有三個CDRs)的重鏈;一種含有SEQ ID NO:8的一或更多CDRs(例如,所有三個CDRs)的輕鏈及一種含有SEQ ID NO:21的一或更多CDRs(例如,所有三個CDRs)的重鏈;一種含有SEQ ID NO:9的一或更多CDRs(例如,所有三個CDRs)的輕鏈及一種含有SEQ ID NO:22的一或更多CDRs(例如,所有三個CDRs)的重鏈;一種含有SEQ ID NO:10的一或更多CDRs(例如,所有三個CDRs)的輕鏈及一種含有SEQ ID NO:23的一或更多CDRs(例如,所有三個CDRs)的重鏈;一種含有SEQ ID NO:11的一或更多CDRs(例如,所有三個CDRs)的輕鏈及一種含有SEQ ID NO:24的一或更多CDRs(例如,所有三個CDRs)的重鏈;一種含有SEQ ID NO:12的一或更多CDRs(例如,所有三個CDRs)的輕鏈及一種含有SEQ ID NO:25的一或更多CDRs(例如,所有三個CDRs)的重鏈;一種含有SEQ ID NO:12的一或更多CDRs(例如,所有三個CDRs)的輕鏈及一種含有SEQ ID NO:137的一或更多CDRs(例如,所有三個CDRs)的重鏈;或是一種含有SEQ ID NO:13的一或更多CDRs(例如,所有三個CDRs)的輕鏈及一種含有SEQ ID NO:26的一或更多CDRs(例如,所有三個CDRs)的重鏈。在上文所提及SEQ ID NOs的CDRs係由第1及2圖表示及參考此處所提供表1-6。The humanized immunoglobulins described herein can comprise a humanized heavy chain and a humanized light chain. In a specific embodiment, the humanized immunoglobulin comprises a light chain comprising one or more CDRs of SEQ ID NO: 3 (eg, all three CDRs) and one or more CDRs comprising SEQ ID NO: a heavy chain (eg, all three CDRs); a light chain comprising one or more CDRs of SEQ ID NO: 4 (eg, all three CDRs) and one or more CDRs comprising SEQ ID NO: a heavy chain (eg, all three CDRs); a light chain comprising one or more CDRs of SEQ ID NO: 5 (eg, all three CDRs) and one or more CDRs comprising SEQ ID NO: 18. a heavy chain (eg, all three CDRs); a light chain comprising one or more CDRs of SEQ ID NO: 6 (eg, all three CDRs) and one or more CDRs comprising SEQ ID NO: Heavy chain; a light chain comprising one or more CDRs of SEQ ID NO: 7 (eg, all three CDRs) and one or more CDRs comprising SEQ ID NO: 20 (eg, all three CDRs) Heavy chain; a light chain comprising one or more CDRs of SEQ ID NO: 8 (eg, all three CDRs) and one or more CDRs comprising SEQ ID NO: 21 (eg, all three CDRs) of a chain; a light chain comprising one or more CDRs of SEQ ID NO: 9 (eg, all three CDRs) and a heavy chain comprising one or more CDRs of SEQ ID NO: 22 (eg, all three CDRs) a chain; a light chain comprising one or more CDRs of SEQ ID NO: 10 (eg, all three CDRs) and a heavy chain comprising one or more CDRs of SEQ ID NO: 23 (eg, all three CDRs) a chain; a light chain comprising one or more CDRs of SEQ ID NO: 11 (eg, all three CDRs) and a heavy chain comprising one or more CDRs of SEQ ID NO: 24 (eg, all three CDRs) a chain; a light chain comprising one or more CDRs of SEQ ID NO: 12 (eg, all three CDRs) and a heavy chain comprising one or more CDRs of SEQ ID NO: 25 (eg, all three CDRs) a chain; a light chain comprising one or more CDRs of SEQ ID NO: 12 (eg, all three CDRs) and a heavy chain comprising one or more CDRs of SEQ ID NO: 137 (eg, all three CDRs) a chain; or a light chain comprising one or more CDRs of SEQ ID NO: 13 (eg, all three CDRs) and one or more CDRs comprising SEQ ID NO: 26 (eg, all three CDRs) Heavy chain. The CDRs of SEQ ID NOs referred to above are represented by Figures 1 and 2 and with reference to Tables 1-6 provided herein.

在另一具體實施例,具人類CD52結合專一性的人類化免疫球蛋白包含一種輕鏈,其包含由SEQ ID NO:27、SEQ ID NO:28、SEQ ID NO:29、SEQ ID NO:30、SEQ ID NO:31、SEQ ID NO:32、SEQ ID NO:33、SEQ ID NO:34、SEQ ID NO:35、SEQ ID NO:36、SEQ ID NO:37、SEQ ID NO:38、SEQ ID NO:39、SEQ ID NO:40、SEQ ID NO:41、SEQ ID NO:42、SEQ ID NO:43、SEQ ID NO:44、SEQ ID NO:45、SEQ ID NO:46、SEQ ID NO:47、及SEQ ID NO:48所組成的群組中選出的一或更多CDRs(例如,所有三個);一種重鏈,其包含由SEQ ID NO:49、SEQ ID NO:50、SEQ ID NO:51、SEQ ID NO:52、SEQ ID NO:53、SEQ ID NO:54、SEQ ID NO:55、SEQ ID NO:56、SEQ ID NO:57、SEQ ID NO:58、SEQ ID NO:59、SEQ ID NO:60、SEQ ID NO:61、SEQ ID NO:62、SEQ ID NO:63、SEQ ID NO:64、SEQ ID NO:65、SEQ ID NO:66、SEQ ID NO:67、SEQ ID NO:68、SEQ ID NO:69、SEQ ID NO:70、SEQ ID NO:71、SEQ ID NO:72、SEQ ID NO:73、SEQ ID NO:74、及SEQ ID NO: 294所組成的群組中選出的一或更多CDRs(例如,所有三個);或是此種輕鏈及此種重鏈;其中該人類化免疫球蛋白不為CampathIn another embodiment, a humanized immunoglobulin having human CD52 binding specificity comprises a light chain comprising SEQ ID NO:27, SEQ ID NO:28, SEQ ID NO:29, SEQ ID NO:30 SEQ ID NO: 31, SEQ ID NO: 32, SEQ ID NO: 33, SEQ ID NO: 34, SEQ ID NO: 35, SEQ ID NO: 36, SEQ ID NO: 37, SEQ ID NO: 38, SEQ ID NO: 39, SEQ ID NO: 40, SEQ ID NO: 41, SEQ ID NO: 42, SEQ ID NO: 43, SEQ ID NO: 44, SEQ ID NO: 45, SEQ ID NO: 46, SEQ ID NO : 47, and one or more CDRs (eg, all three) selected from the group consisting of SEQ ID NO: 48; a heavy chain comprising SEQ ID NO: 49, SEQ ID NO: 50, SEQ ID NO: 51, SEQ ID NO: 52, SEQ ID NO: 53, SEQ ID NO: 54, SEQ ID NO: 55, SEQ ID NO: 56, SEQ ID NO: 57, SEQ ID NO: 58, SEQ ID NO :59, SEQ ID NO: 60, SEQ ID NO: 61, SEQ ID NO: 62, SEQ ID NO: 63, SEQ ID NO: 64, SEQ ID NO: 65, SEQ ID NO: 66, SEQ ID NO: 67 SEQ ID NO: 68, SEQ ID NO: 69, SEQ ID NO: 70, SEQ ID NO: 71, SEQ ID NO: 72, SEQ ID NO: 73, SEQ ID NO: 74, and SEQ ID NO: 294 One or more CDRs selected from the group consisting of As all three); or such and such a heavy chain light chain; wherein the humanized immunoglobulin is not Campath .

在另一具體實施例,具人類CD52結合專一性的人類化免疫球蛋白包含一種輕鏈,其包含SEQ ID NO:3、SEQ ID NO:4、SEQ ID NO:5、SEQ ID NO:6、SEQ ID NO:7、SEQ ID NO:8、SEQ ID NO:9、SEQ ID NO:10、SEQ ID NO:11、SEQ ID NO:12、或SEQ ID NO:13的一或更多CDRs(例如,所有三個CDRs);一種重鏈,其包含SEQ ID NO:16、SEQ ID NO:17、SEQ ID NO:18、SEQ ID NO:19、SEQ ID NO:20、SEQ ID NO:21、SEQ ID NO:22、SEQ ID NO:23、SEQ ID NO:24、SEQ ID NO:25、SEQ ID NO:26、或SEQ ID NO:137的一或更多CDRs(例如,所有三個CDRs);或是此種輕鏈及此種重鏈;其中該人類化免疫球蛋白不為CampathIn another embodiment, the humanized immunoglobulin having human CD52 binding specificity comprises a light chain comprising SEQ ID NO:3, SEQ ID NO:4, SEQ ID NO:5, SEQ ID NO:6, One or more CDRs of SEQ ID NO: 7, SEQ ID NO: 8, SEQ ID NO: 9, SEQ ID NO: 10, SEQ ID NO: 11, SEQ ID NO: 12, or SEQ ID NO: 13 (eg, , all three CDRs); a heavy chain comprising SEQ ID NO: 16, SEQ ID NO: 17, SEQ ID NO: 18, SEQ ID NO: 19, SEQ ID NO: 20, SEQ ID NO: 21, SEQ ID NO: 22, SEQ ID NO: 23, SEQ ID NO: 24, SEQ ID NO: 25, SEQ ID NO: 26, or one or more CDRs of SEQ ID NO: 137 (eg, all three CDRs); Or such a light chain and such a heavy chain; wherein the human immunoglobulin is not Campath .

在一些具體實施例,人類化免疫球蛋白的骨架區具與一種免疫球蛋白(由此得到輕鏈CDRs及重鏈CDRs)骨架區的至少50%同源性。例如,人類化免疫球蛋白的骨架區可與生殖細胞系的人類免疫球蛋白序列至少50%,至少60%,至少70%,至少80%,至少90%,至少95%,至少98%,至少99%,或甚至100%相同。在一個具體實施例,人類化免疫球蛋白的骨架區可自IgG人類抗體變異區得到或衍生。在另一具體實施例,CD52為野生型人類CD52。在另一具體實施例,人類化免疫球蛋白可與阿來組單抗(alemtuzumab)競爭以結合至人類CD52,例如,其可結合至與阿來組單抗所要結合的抗原決定區相同的抗原決定區,或是與之重疊的抗原決定區。In some embodiments, the framework region of the humanized immunoglobulin has at least 50% homology to the framework region of an immunoglobulin (and thus the light chain CDRs and heavy chain CDRs). For example, the framework region of the humanized immunoglobulin can be at least 50%, at least 60%, at least 70%, at least 80%, at least 90%, at least 95%, at least 98%, at least at least 60%, at least 98%, at least 98% of the human immunoglobulin sequence of the germ cell line. 99%, or even 100% identical. In a specific embodiment, the framework region of the humanized immunoglobulin can be obtained or derived from an IgG human antibody variant region. In another specific embodiment, CD52 is wild-type human CD52. In another embodiment, the humanized immunoglobulin can compete with alemtuzumab for binding to human CD52, for example, it can bind to the same antigen as the epitope determined to bind to alemtuzumab. Determine the area, or the antigenic decision area that overlaps it.

本發明亦相關於本發明人類化免疫球蛋白的人類化輕鏈。在一個具體實施例,人類化輕鏈包含由SEQ ID NO:27、SEQ ID NO:28、SEQ ID NO:29、SEQ ID NO:30、SEQ ID NO:31、SEQ ID NO:32、SEQ ID NO:33、SEQ ID NO:34、SEQ ID NO:35、SEQ ID NO:36、SEQ ID NO:37、SEQ ID NO:38、SEQ ID NO:39、SEQ ID NO:40、SEQ ID NO:41、SEQ ID NO:42、SEQ ID NO:43、SEQ ID NO:44、SEQ ID NO:45、SEQ ID NO:46、SEQ ID NO:47、及SEQ ID NO:48所組成的群組中選出的一或更多CDRs或是其組合,其中該人類化輕鏈不為Campath的人類化輕鏈。The invention is also related to the humanized light chain of the humanized immunoglobulin of the invention. In a specific embodiment, the humanized light chain comprises SEQ ID NO:27, SEQ ID NO:28, SEQ ID NO:29, SEQ ID NO:30, SEQ ID NO:31, SEQ ID NO:32, SEQ ID NO: 33, SEQ ID NO: 34, SEQ ID NO: 35, SEQ ID NO: 36, SEQ ID NO: 37, SEQ ID NO: 38, SEQ ID NO: 39, SEQ ID NO: 40, SEQ ID NO: 41. In the group consisting of SEQ ID NO: 42, SEQ ID NO: 43, SEQ ID NO: 44, SEQ ID NO: 45, SEQ ID NO: 46, SEQ ID NO: 47, and SEQ ID NO: 48 One or more selected CDRs or a combination thereof, wherein the humanized light chain is not Campath Humanized light chain.

在另一具體實施例,人類化輕鏈包含SEQ ID NO:3、SEQ ID NO:4、SEQ ID NO:5、SEQ ID NO:6、SEQ ID NO:7、SEQ ID NO:8、SEQ ID NO:9、SEQ ID NO:10、SEQ ID NO:11、SEQ ID NO:12或SEQ ID NO:13的一或更多CDRs(例如,所有三個CDRs),其中該人類化輕鏈不為Campath的人類化輕鏈。In another specific embodiment, the humanized light chain comprises SEQ ID NO:3, SEQ ID NO:4, SEQ ID NO:5, SEQ ID NO:6, SEQ ID NO:7, SEQ ID NO:8, SEQ ID NO: 9, one or more CDRs of SEQ ID NO: 10, SEQ ID NO: 11, SEQ ID NO: 12 or SEQ ID NO: 13 (eg, all three CDRs), wherein the humanized light chain is not Campath Humanized light chain.

本發明亦相關於本發明人類化免疫球蛋白的人類化重鏈。在一個具體實施例,人類化重鏈包含由SEQ ID NO:49、SEQ ID NO:50、SEQ ID NO:51、SEQ ID NO:52、SEQ ID NO:53、SEQ ID NO:54、SEQ ID NO:55、SEQ ID NO:56、SEQ ID NO:57、SEQ ID NO:58、SEQ ID NO:59、SEQ ID NO:60、SEQ ID NO:61、SEQ ID NO:62、SEQ ID NO:63、SEQ ID NO:64、SEQ ID NO:65、SEQ ID NO:66、SEQ ID NO:67、SEQ ID NO:68、SEQ ID NO:69、SEQ ID NO:70、SEQ ID NO:71、SEQ ID NO:72、SEQ ID NO:73、SEQ ID NO:74、及SEQ ID NO: 294所組成的群組中選出的Ig變異區的一或更多CDRs,或是其組合,其中該人類化重鏈不為Campath的人類化重鏈。The invention is also related to the humanized heavy chain of the humanized immunoglobulin of the invention. In a specific embodiment, the humanized heavy chain comprises SEQ ID NO:49, SEQ ID NO:50, SEQ ID NO:51, SEQ ID NO:52, SEQ ID NO:53, SEQ ID NO:54, SEQ ID NO: 55, SEQ ID NO: 56, SEQ ID NO: 57, SEQ ID NO: 58, SEQ ID NO: 59, SEQ ID NO: 60, SEQ ID NO: 61, SEQ ID NO: 62, SEQ ID NO: 63, SEQ ID NO: 64, SEQ ID NO: 65, SEQ ID NO: 66, SEQ ID NO: 67, SEQ ID NO: 68, SEQ ID NO: 69, SEQ ID NO: 70, SEQ ID NO: 71, One or more CDRs of the Ig variant region selected from the group consisting of SEQ ID NO: 72, SEQ ID NO: 73, SEQ ID NO: 74, and SEQ ID NO: 294, or a combination thereof, wherein the human Heavy chain is not for Campath Humanized heavy chain.

在另一具體實施例,人類化重鏈包含SEQ ID NO:16、SEQ ID NO:17、SEQ ID NO:18、SEQ ID NO:19、SEQ ID NO:20、SEQ ID NO:21、SEQ ID NO:22、SEQ ID NO:23、SEQ ID NO:24、SEQ ID NO:25、SEQ ID NO:26、或SEQ ID NO:137的一或更多CDRs(例如,所有三個CDRs);其中該人類化重鏈不為Campath的人類化重鏈。In another embodiment, the humanized heavy chain comprises SEQ ID NO: 16, SEQ ID NO: 17, SEQ ID NO: 18, SEQ ID NO: 19, SEQ ID NO: 20, SEQ ID NO: 21, SEQ ID NO: 22. One or more CDRs of SEQ ID NO: 23, SEQ ID NO: 24, SEQ ID NO: 25, SEQ ID NO: 26, or SEQ ID NO: 137 (eg, all three CDRs); The humanized heavy chain is not for Campath Humanized heavy chain.

較佳為,本發明人類化免疫球蛋白包含本發明人類化輕鏈及本發明人類化重鏈。Preferably, the humanized immunoglobulin of the present invention comprises the humanized light chain of the present invention and the humanized heavy chain of the present invention.

在其他具體實施例,本發明係提供一種結合至人類CD52上的抗原決定區的人類化免疫球蛋白,該抗原決定區與老鼠單株抗體所結合的相同抗原決定區或是與之競爭或交叉競爭於,該老鼠單株抗體包含SEQ ID NO: 3的輕鏈變異區及SEQ ID NO: 16的重鏈變異區;SEQ ID NO: 4的輕鏈變異區及SEQ ID NO: 17的重鏈變異區;SEQ ID NO: 5的輕鏈變異區及SEQ ID NO: 18的重鏈變異區;SEQ ID NO: 6的輕鏈變異區及SEQ ID NO: 19的重鏈變異區;SEQ ID NO: 7的輕鏈變異區及SEQ ID NO: 20的重鏈變異區;SEQ ID NO: 8的輕鏈變異區及SEQ ID NO: 21的重鏈變異區;SEQ ID NO: 9的輕鏈變異區及SEQ ID NO: 22的重鏈變異區;SEQ ID NO: 10的輕鏈變異區及SEQ ID NO: 23的重鏈變異區;SEQ ID NO: 11的輕鏈變異區及SEQ ID NO: 24的重鏈變異區;SEQ ID NO: 12的輕鏈變異區及SEQ ID NO: 25的重鏈變異區;或是SEQ ID NO: 13的輕鏈變異區及SEQ ID NO: 26的重鏈變異區。在其他具體實施例,人類化免疫球蛋白結合至人類CD52上的抗原決定區,其與老鼠單株抗體所結合的抗原決定區重疊。In other embodiments, the invention provides a humanized immunoglobulin that binds to an epitope of human CD52 that competes with or crosses the same epitope associated with a mouse monoclonal antibody. In competition, the mouse monoclonal antibody comprises the light chain variant region of SEQ ID NO: 3 and the heavy chain variant region of SEQ ID NO: 16; the light chain variant region of SEQ ID NO: 4 and the heavy chain of SEQ ID NO: Variant region; light chain variant region of SEQ ID NO: 5 and heavy chain variant region of SEQ ID NO: 18; light chain variant region of SEQ ID NO: 6 and heavy chain variant region of SEQ ID NO: 19; SEQ ID NO a light chain variant region of 7 and a heavy chain variant region of SEQ ID NO: 20; a light chain variant region of SEQ ID NO: 8 and a heavy chain variant region of SEQ ID NO: 21; light chain variation of SEQ ID NO: a region and a heavy chain variant region of SEQ ID NO: 22; a light chain variant region of SEQ ID NO: 10 and a heavy chain variant region of SEQ ID NO: 23; a light chain variant region of SEQ ID NO: 11 and SEQ ID NO: a heavy chain variant region of 24; a light chain variant region of SEQ ID NO: 12 and a heavy chain variant region of SEQ ID NO: 25; or a light chain variant region of SEQ ID NO: 13 and a heavy chain of SEQ ID NO: variation Area. In other embodiments, the humanized immunoglobulin binds to an epitope on human CD52 that overlaps with an epitope determined by the mouse monoclonal antibody.

在其他具體實施例,本發明提供一種結合至人類CD52(例如,SEQ ID NO:104)上的抗原決定區之人類化免疫球蛋白,其包含成熟人類CD52序列的至少殘基1(於此殘基1為成熟人類CD52序列的N-端,亦即,N-端甘胺酸[G]殘基;參考第4圖)。人類化免疫球蛋白可結合至包含成熟人類CD52序列的至少殘基1、3、4及5的抗原決定區(這些殘基分別為甘胺酸[G]、天門冬胺酸[N]、天冬胺酸鹽[D]、及蘇胺酸[T])。人類化免疫球蛋白可結合至包含成熟人類CD52序列的至少殘基1、2、3、4及5的抗原決定區(這些殘基分別為甘胺酸[G]、麩醯胺[Q]、天門冬胺酸[N]、天冬胺酸鹽[D]、及蘇胺酸[T])。在其他具體實施例,本發明係提供一種結合至人類CD52上的抗原決定區之人類化免疫球蛋白,其包含成熟人類CD52序列的至少殘基7、8及9(這些殘基分別為麩醯胺[Q]、蘇胺酸[T]、及絲胺酸[S])。在一些具體實施例,抗原決定區包含成熟人類CD52序列的至少殘基7(Q)、8(T)及11(P)。在一些具體實施例,抗原決定區包含成熟人類CD52序列的至少殘基4(D)及11(P)。In other specific embodiments, the invention provides a humanized immunoglobulin that binds to an epitope of human CD52 (eg, SEQ ID NO: 104) comprising at least residue 1 of a mature human CD52 sequence Base 1 is the N-terminus of the mature human CD52 sequence, that is, the N-terminal glycine [G] residue; see Figure 4). The humanized immunoglobulin can bind to an epitope comprising at least residues 1, 3, 4 and 5 of the mature human CD52 sequence (the residues are glycine [G], aspartic acid [N], day respectively Aspartate [D], and threonine [T]). The humanized immunoglobulin can bind to an epitope comprising at least residues 1, 2, 3, 4 and 5 of the mature human CD52 sequence (the residues are glycine [G], glutamine [Q], respectively) Aspartic acid [N], aspartate [D], and threonine [T]). In other embodiments, the invention provides a humanized immunoglobulin that binds to an epitope of human CD52 comprising at least residues 7, 8 and 9 of the mature human CD52 sequence (the residues are bran Amine [Q], threonine [T], and serine [S]). In some embodiments, the epitope comprises at least residues 7 (Q), 8 (T), and 11 (P) of the mature human CD52 sequence. In some embodiments, the epitope comprises at least residues 4 (D) and 11 (P) of the mature human CD52 sequence.

在一些具體實施例,本發明係提供一種結合至人類CD52的人類化免疫球蛋白,及其包含一種輕鏈,其包含由SEQ ID NO: 115、SEQ ID NO: 118、及SEQ ID NO: 121所組成的群組中選出的一或更多CDRs(例如,所有三個該CDRs),或是一種重鏈,其包含由SEQ ID NO: 124、SEQ ID NO: 127、及SEQ ID NO: 130所組成的群組中選出的一或更多CDRs(例如,所有三個該CDRs),或是此種輕鏈及此種重鏈都有。在其他具體實施例,本發明係提供一種結合至人類CD52的人類化免疫球蛋白,及其包含一種輕鏈,其包含由SEQ ID NO: 116、SEQ ID NO: 119、及SEQ ID NO: 122所組成的群組中選出的一或更多CDRs(例如,所有三個該CDRs),或是一種重鏈,其包含由SEQ ID NO: 125、SEQ ID NO: 128、及SEQ ID NO: 131所組成的群組中選出的一或更多CDRs(例如,所有三個該CDRs),或是此種輕鏈及此種重鏈都有。在進一步具體實施例,本發明係提供一種結合至人類CD52的人類化免疫球蛋白,及其包含一種輕鏈,其包含由SEQ ID NO: 117、SEQ ID NO: 120、及SEQ ID NO: 123所組成的群組中選出的一或更多CDRs(例如,所有三個該CDRs),或是一種重鏈,其包含由SEQ ID NO: 126、SEQ ID NO: 129、及SEQ ID NO: 132所組成的群組中選出的一或更多CDRs(例如,所有三個該CDRs),或是此種輕鏈及此種重鏈都有。In some embodiments, the invention provides a humanized immunoglobulin that binds to human CD52, and comprises a light chain comprising SEQ ID NO: 115, SEQ ID NO: 118, and SEQ ID NO: 121 One or more CDRs (eg, all three of the CDRs) selected from the group consisting of, or a heavy chain comprising SEQ ID NO: 124, SEQ ID NO: 127, and SEQ ID NO: 130 One or more CDRs (for example, all three of the CDRs) selected from the group consisting of, or such a light chain and such a heavy chain. In other specific embodiments, the invention provides a humanized immunoglobulin that binds to human CD52, and comprises a light chain comprising SEQ ID NO: 116, SEQ ID NO: 119, and SEQ ID NO: 122 One or more CDRs (eg, all three of the CDRs) selected from the group consisting of, or a heavy chain comprising SEQ ID NO: 125, SEQ ID NO: 128, and SEQ ID NO: 131 One or more CDRs (for example, all three of the CDRs) selected from the group consisting of, or such a light chain and such a heavy chain. In a further embodiment, the invention provides a humanized immunoglobulin that binds to human CD52, and comprises a light chain comprising SEQ ID NO: 117, SEQ ID NO: 120, and SEQ ID NO: 123 One or more CDRs (eg, all three of the CDRs) selected from the group consisting of, or a heavy chain comprising SEQ ID NO: 126, SEQ ID NO: 129, and SEQ ID NO: 132 One or more CDRs (for example, all three of the CDRs) selected from the group consisting of, or such a light chain and such a heavy chain.

在某些具體實施例,人類化免疫球蛋白包含一種輕鏈,其包含SEQ ID NO: 115、SEQ ID NO: 118及SEQ ID NO: 121的CDRs及一種重鏈,其包含SEQ ID NO: 124、SEQ ID NO: 127及SEQ ID NO: 130的CDRs。在其他具體實施例,人類化免疫球蛋白包含一種輕鏈,其包含SEQ ID NO: 116、SEQ ID NO: 119及SEQ ID NO: 122的CDRs及一種重鏈,其包含SEQ ID NO: 125、SEQ ID NO: 128及SEQ ID NO: 131的CDRs。在其他具體實施例,人類化免疫球蛋白包含一種輕鏈,其包含SEQ ID NO: 117、SEQ ID NO: 120及SEQ ID NO: 123的CDRs及一種重鏈,其包含SEQ ID NO: 126、SEQ ID NO: 129及SEQ ID NO: 132的CDRs。In certain embodiments, the humanized immunoglobulin comprises a light chain comprising the CDRs of SEQ ID NO: 115, SEQ ID NO: 118 and SEQ ID NO: 121, and a heavy chain comprising SEQ ID NO: 124 CDRs of SEQ ID NO: 127 and SEQ ID NO: 130. In other embodiments, the humanized immunoglobulin comprises a light chain comprising the CDRs of SEQ ID NO: 116, SEQ ID NO: 119, and SEQ ID NO: 122, and a heavy chain comprising SEQ ID NO: 125, CDRs of SEQ ID NO: 128 and SEQ ID NO: 131. In other embodiments, the human immunoglobulin comprises a light chain comprising CDRs of SEQ ID NO: 117, SEQ ID NO: 120 and SEQ ID NO: 123, and a heavy chain comprising SEQ ID NO: 126, CDRs of SEQ ID NO: 129 and SEQ ID NO: 132.

本發明人類化免疫球蛋白係與人類化免疫球蛋白Campath不同。Humanized immunoglobulin system and humanized immunoglobulin Campath of the present invention different.

上文所提及SEQ ID NOs: 115-132的肽基酸序列係提供於下文,及係基於在本文他處所提供的表1-6所報告的胺基酸序列。在這些胺基酸序列,「X」表示任何胺基酸,及符號「/」表示相臨該符號的胺基酸其中一個(或任何胺基酸)可存在於所指出位置(例如,K/R表示離胺酸或精胺酸殘基係存在於所指出位置及F/L/V指出苯丙胺酸丙胺酸、白胺酸白胺酸或纈胺酸殘基係存在於所指出位置)。The peptidic acid sequences of SEQ ID NOs: 115-132 referred to above are provided below, and are based on the amino acid sequences reported in Tables 1-6 provided elsewhere herein. In these amino acid sequences, "X" means any amino acid, and the symbol "/" means that one of the amino acids adjacent to the symbol (or any amino acid) may be present at the indicated position (for example, K/). R indicates that the amino acid or arginine residue is present at the indicated position and F/L/V indicates that the amphetamine, leucine or valine acid residues are present at the indicated positions).

輕鏈CDR-1序列Light chain CDR-1 sequence

K/RSSQSLL/V/IXS/TN/DGXS/TYLX(SEQ ID NO:115)K/RSSQSLL/V/IXS/TN/DGXS/TYLX (SEQ ID NO: 115)

K/RSSQSLL/V/IHS/TNGXS/TYLH(SEQ ID NO:116)K/RSSQSLL/V/IHS/TNGXS/TYLH (SEQ ID NO: 116)

RSSQSLVHTNGNS/TYLH(SEQ ID NO:117)RSSQSLVHTNGNS/TYLH (SEQ ID NO: 117)

輕鏈CDR-2序列Light chain CDR-2 sequence

XVSXXXS(SEQ ID NO:118)XVSXXXS (SEQ ID NO: 118)

XVSXRXS(SEQ ID NO:119)XVSXRXS (SEQ ID NO: 119)

MVSXRFS(SEQ ID NO:120)MVSXRFS (SEQ ID NO: 120)

輕鏈CDR-3序列Light chain CDR-3 sequence

XQXXH/R/KF/L/V/IXX(SEQ ID NO:121)XQXXH/R/KF/L/V/IXX (SEQ ID NO: 121)

SQSXH/R/KF/L/V/IPX(SEQ ID NO:122)SQSXH/R/KF/L/V/IPX (SEQ ID NO: 122)

SQSXHVPF/P(SEQ ID NO:123)SQSXHVPF/P (SEQ ID NO: 123)

重鏈CDR-1序列Heavy chain CDR-1 sequence

GFXFXXYW/YMX(SEQ ID NO:124)GFXFXXYW/YMX (SEQ ID NO: 124)

GFTFXXYW/YMX(SEQ ID NO:125)GFTFXXYW/YMX (SEQ ID NO: 125)

GFTFTDYW/YMS(SEQ ID NO:126)GFTFTDYW/YMS (SEQ ID NO: 126)

重鏈CDR-2序列Heavy chain CDR-2 sequence

XIRXKXBXYXTXYXXSVKG(SEQ ID NO:127)XIRXKXBXYXTXYXXSVKG (SEQ ID NO: 127)

XIRXKXNXYTTEYXXSVKG(SEQ ID NO:128)XIRXKXNXYTTEYXXSVKG (SEQ ID NO: 128)

FIRNKANGYTTEYXXSVKG(SEQ ID NO:129)FIRNKANGYTTEYXXSVKG (SEQ ID NO: 129)

重鏈CDR-3序列Heavy chain CDR-3 sequence

TXXXY/F/W(SEQ ID NO:130)TXXXY/F/W (SEQ ID NO: 130)

TRYXY/F/WFDY(SEQ ID NO:131)TRYXY/F/WFDY (SEQ ID NO: 131)

TRYIF/WFDY(SEQ ID NO:132)TRYIF/WFDY (SEQ ID NO: 132)

本發明亦相關於一種人類化輕鏈,其包含由SEQ ID NO: 115、SEQ ID NO: 118、及SEQ ID NO: 121所組成的群組中選出的一或更多CDRs(例如,所有三個該CDRs);一種人類化輕鏈,其包含由SEQ ID NO: 116、SEQ ID NO: 119、及SEQ ID NO: 122所組成的群組中選出的一或更多CDRs(例如,所有三個該CDRs);或是一種人類化輕鏈,其包含由SEQ ID NO: 117、SEQ ID NO: 120、及SEQ ID NO: 123所組成的群組中選出的一或更多CDRs(例如,所有三個該CDRs)。The invention also relates to a humanized light chain comprising one or more CDRs selected from the group consisting of SEQ ID NO: 115, SEQ ID NO: 118, and SEQ ID NO: 121 (eg, all three One such CDRs); a humanized light chain comprising one or more CDRs selected from the group consisting of SEQ ID NO: 116, SEQ ID NO: 119, and SEQ ID NO: 122 (eg, all three) One such CDRs); or a humanized light chain comprising one or more CDRs selected from the group consisting of SEQ ID NO: 117, SEQ ID NO: 120, and SEQ ID NO: 123 (eg, All three of these CDRs).

本發明亦相關於一種人類化重鏈,其包含由SEQ ID NO: 124、SEQ ID NO: 127、及SEQ ID NO: 130所組成的群組中選出的一或更多CDRs(例如,所有三個該CDRs);一種人類化重鏈,其包含由SEQ ID NO: 125、SEQ ID NO:128、及SEQ ID NO: 131所組成的群組中選出的一或更多CDRs(例如,所有三個該CDRs);或是一種人類化重鏈,其包含由SEQ ID NO: 126、SEQ ID NO: 129、及SEQ ID NO: 132所組成的群組中選出的一或更多CDRs(例如,所有三個該CDRs)。The invention also relates to a humanized heavy chain comprising one or more CDRs selected from the group consisting of SEQ ID NO: 124, SEQ ID NO: 127, and SEQ ID NO: 130 (eg, all three The CDRs); a humanized heavy chain comprising one or more CDRs selected from the group consisting of SEQ ID NO: 125, SEQ ID NO: 128, and SEQ ID NO: 131 (eg, all three) One such CDRs); or a humanized heavy chain comprising one or more CDRs selected from the group consisting of SEQ ID NO: 126, SEQ ID NO: 129, and SEQ ID NO: 132 (eg, All three of these CDRs).

本發明人類化輕鏈及人類化重鏈與人類化免疫球蛋白Campath的人類化輕鏈及人類化重鏈不同。Humanized light chain and humanized heavy chain of the invention and humanized immunoglobulin Campath The humanized light chain and the humanized heavy chain are different.

在一些本發明具體實施例,本發明的人類化免疫球蛋白(無論可能另外定義的方式,例如,無論它們是否亦以一或更多CDRs的順序定義及/或藉由與老鼠單株抗體或是另一人類化免疫球蛋白的交叉反應性的方式定義):(1)顯現對於結合至醣化及去醣化CD52沒有任何明顯偏好;(2)顯現對醣化CD52的結合專一性;(3)顯現對去醣化CD52的結合專一性;或(4)相較於醣化CD52顯現對去-醣化的結合偏好。在某些具體實施例,本發明的人類化免疫球蛋白對醣化人類CD52較對非-醣化或去-醣化人類CD52具有更大結合親和力。的確,在某些本發明的具體實施例,本發明人類化免疫球蛋白顯現對醣化人類CD52特定的結合。對非-醣化或去-醣化人類CD52的結合親和力可使用醣苷酶,例如使用內切醣苷酶PNGase-F,將成熟人類CD52去醣化來測定。在某些本發明具體實施例,本發明的人類化免疫球蛋白結合至包含其N-鍵結碳水化合物基團的成熟人類CD52上的抗原決定區。此碳水化合物基團為一種唾液酸化,含聚乳糖胺核心岩藻糖四天線N-鍵結的低聚糖(Treumann,A.等.,(1995) J. Biol. Chem. 270:6088-6099)。此抗原決定區亦可包含至少成熟人類CD52序列的殘基1,至少成熟人類CD52序列的殘基3,至少成熟人類CD52序列的殘基1、3、4及5,或是至少成熟人類CD52序列的殘基1、2、3、4及5。在一些具體實施例,本發明老鼠或嵌合抗體可具任何這些結合特徵。In some embodiments of the invention, humanized immunoglobulins of the invention (whether or not otherwise defined, for example, whether or not they are also defined in the order of one or more CDRs and/or by antibodies to mouse monoclonal antibodies or Is another way to define the cross-reactivity of human immunoglobulins): (1) appears to have no obvious preference for binding to glycosylated and de-glycosylated CD52; (2) exhibits binding specificity for glycosylated CD52; (3) appears Binding specificity for de-saccharified CD52; or (4) exhibits binding preference for de-saccharification compared to glycated CD52. In certain embodiments, the humanized immunoglobulins of the invention have greater binding affinity for glycosylated human CD52 than for non-glycated or de-glycosylated human CD52. Indeed, in certain embodiments of the invention, the humanized immunoglobulins of the invention exhibit specific binding to glycosylated human CD52. The binding affinity for non-glycated or de-glycosylated human CD52 can be determined using a glycosidase, for example, using the endoglycosidase PNGase-F to de-saccharify mature human CD52. In certain embodiments of the invention, the humanized immunoglobulin of the invention binds to an epitope on mature human CD52 comprising its N -bonded carbohydrate group. This carbohydrate group is a sialylated, oligosaccharide containing a polylactosamine core fucose four-antenna N -bond (Treumann, A. et al., (1995) J. Biol. Chem . 270: 6088-6099 ). The epitope may also comprise at least residue 1 of the mature human CD52 sequence, at least residue 3 of the mature human CD52 sequence, at least residues 1, 3, 4 and 5 of the mature human CD52 sequence, or at least the mature human CD52 sequence. Residues 1, 2, 3, 4 and 5. In some embodiments, the mouse or chimeric antibody of the invention can have any of these binding characteristics.

亦提供編碼本發明人類化免疫球蛋白、人類化輕鏈或人類化重鏈的經分離核酸分子,如在本文他處所定義。在一些具體實施例,本發明為一種(一或更多)經分離核酸分子,其編碼人類化輕鏈及人類化重鏈(其在一起會形成具有對人類CD52的結合專一性的人類化免疫球蛋白),其中人類化輕鏈包含SEQ ID NO: 3的一或更多CDRs(例如,所有三個CDRs)及包含SEQ ID NO: 16的一或更多CDRs(例如,所有三個CDRs)的重鏈;包含SEQ ID NO:4的一或更多CDRs(例如,所有三個CDRs)的輕鏈及包含SEQ ID NO:17的一或更多CDRs(例如,所有三個CDRs)的重鏈;包含SEQ ID NO:5的一或更多CDRs(例如,所有三個CDRs)的輕鏈及包含SEQ ID NO:18的一或更多CDRs(例如,所有三個CDRs)的重鏈;包含SEQ ID NO:6的一或更多CDRs(例如,所有三個CDRs)的輕鏈及包含SEQ ID NO:19的一或更多CDRs(例如,所有三個CDRs)的重鏈;包含SEQ ID NO:7的一或更多CDRs(例如,所有三個CDRs)的輕鏈及包含SEQ ID NO:20的一或更多CDRs(例如,所有三個CDRs)的重鏈;包含SEQ ID NO:8的一或更多CDRs(例如,所有三個CDRs)的輕鏈及包含SEQ ID NO:21的一或更多CDRs(例如,所有三個CDRs)的重鏈;包含SEQ ID NO:9的一或更多CDRs(例如,所有三個CDRs)的輕鏈及包含SEQ ID NO:22的一或更多CDRs(例如,所有三個CDRs)的重鏈;包含SEQ ID NO:10的一或更多CDRs(例如,所有三個CDRs)的輕鏈及包含SEQ ID NO:23的一或更多CDRs(例如,所有三個CDRs)的重鏈;包含SEQ ID NO:11的一或更多CDRs(例如,所有三個CDRs)的輕鏈及包含SEQ ID NO:24的一或更多CDRs(例如,所有三個CDRs)的重鏈;包含SEQ ID NO:12的一或更多CDRs(例如,所有三個CDRs)的輕鏈及包含SEQ ID NO:25的一或更多CDRs(例如,所有三個CDRs)的重鏈;包含SEQ ID NO:12的一或更多CDRs(例如,所有三個CDRs)的輕鏈及包含SEQ ID NO:137的一或更多CDRs(例如,所有三個CDRs)的重鏈;或是包含SEQ ID NO:13的一或更多CDRs(例如,所有三個CDRs)的輕鏈及包含SEQ ID NO:26的一或更多CDRs(例如,所有三個CDRs)的重鏈序列。Isolated nucleic acid molecules encoding humanized immunoglobulins, humanized light chains or humanized heavy chains of the invention are also provided, as defined elsewhere herein. In some embodiments, the invention is a (one or more) isolated nucleic acid molecule encoding a humanized light chain and a humanized heavy chain (which together form a humanized immunity with binding specificity for human CD52) a globulin), wherein the humanized light chain comprises one or more CDRs of SEQ ID NO: 3 ( eg , all three CDRs) and one or more CDRs comprising SEQ ID NO: 16 ( eg , all three CDRs) Heavy chain; light chain comprising one or more CDRs of SEQ ID NO: 4 ( eg , all three CDRs) and one or more CDRs comprising SEQ ID NO: 17 ( eg , all three CDRs) a chain; a light chain comprising one or more CDRs of SEQ ID NO: 5 ( eg , all three CDRs) and a heavy chain comprising one or more CDRs of SEQ ID NO: 18 ( eg , all three CDRs); a light chain comprising one or more CDRs of SEQ ID NO: 6 ( eg , all three CDRs) and a heavy chain comprising one or more CDRs of SEQ ID NO: 19 ( eg , all three CDRs); comprising SEQ ID NO: one or more CDRs 7 (e.g., all three CDRs) and a light chain comprising SEQ ID NO: one or more CDRs (e.g., all three CDRs) of the heavy chain 20; comprising SEQ ID NO : One or more CDRs 8 (e.g., all three CDRs) and a light chain comprising SEQ ID NO: 21 one or more of the CDRs (e.g., all three CDRs) of the heavy chain; comprising SEQ ID NO: of. 9 one or more CDRs (e.g., all three CDRs) and a light chain comprising SEQ ID NO: 22 one or more of the CDRs (e.g., all three CDRs) of the heavy chain; comprising SEQ ID NO: 10 or a more CDRs (e.g., all three CDRs) and a light chain comprising SEQ ID NO: one or more CDRs 23 (e.g., all three CDRs) of the heavy chain; comprising SEQ ID NO: 11 one or more of CDRs (e.g., all three CDRs) and a light chain comprising SEQ ID NO: one or more CDRs 24 (e.g., all three CDRs) of the heavy chain; comprising SEQ ID NO: 12 one or more of the CDRs ( For example , a light chain of all three CDRs) and a heavy chain comprising one or more CDRs of SEQ ID NO: 25 ( eg , all three CDRs); comprising one or more CDRs of SEQ ID NO: 12 ( eg , a light chain of all three CDRs) and a heavy chain comprising one or more CDRs of SEQ ID NO: 137 ( eg , all three CDRs); or one or more CDRs comprising SEQ ID NO: 13 ( eg , Light chain of all three CDRs) and comprising SEQ ID NO:26 Or more CDRs (e.g., all three CDRs) of the heavy chain sequence.

在一些具體實施例,本發明為一種一或更多經分離核酸分子,其編碼人類化重鏈及人類化輕鏈(其在一起會形成具對人類CD52的特定結合的人類化免疫球蛋白),其中該人類化免疫球蛋白結合至與老鼠單株抗體相同的位於人類CD52之抗原決定區,其包含SEQ ID NO: 3的輕鏈變異區及SEQ ID NO: 16的重鏈變異區;SEQ ID NO: 4的輕鏈變異區及SEQ ID NO: 17的重鏈變異區;SEQ ID NO: 5的輕鏈變異區及SEQ ID NO: 18的重鏈變異區;SEQ ID NO: 6的輕鏈變異區及SEQ ID NO: 19的重鏈變異區;SEQ ID NO: 7的輕鏈變異區及SEQ ID NO: 20的重鏈變異區;SEQ ID NO: 8的輕鏈變異區及SEQ ID NO: 21的重鏈變異區;SEQ ID NO: 9的輕鏈變異區及SEQ ID NO: 22的重鏈變異區;SEQ ID NO: 10的輕鏈變異區及SEQ ID NO: 23的重鏈變異區;SEQ ID NO: 11的輕鏈變異區及SEQ ID NO: 24的重鏈變異區;SEQ ID NO: 12的輕鏈變異區及SEQ ID NO: 25的重鏈變異區;或是SEQ ID NO: 13的輕鏈變異區及SEQ ID NO: 26的重鏈變異區。在其他具體實施例,本發明為一種一或更多經分離核酸分子,其編碼人類化重鏈及人類化輕鏈(其關聯在一起而形成具對人類CD52的特定結合的人類化免疫球蛋白),其中該人類化免疫球蛋白結合至於人類CD52上的抗原決定區,此抗原決定區與老鼠單株抗體所結合的抗原決定區重疊。In some embodiments, the invention is one or more isolated nucleic acid molecules encoding a humanized heavy chain and a humanized light chain (which together form a humanized immunoglobulin having a specific binding to human CD52) Wherein the humanized immunoglobulin binds to the epitope of human CD52 identical to the mouse monoclonal antibody, comprising the light chain variant region of SEQ ID NO: 3 and the heavy chain variant region of SEQ ID NO: 16; ID NO: 4 light chain variant region and heavy chain variant region of SEQ ID NO: 17; light chain variant region of SEQ ID NO: 5 and heavy chain variant region of SEQ ID NO: 18; light of SEQ ID NO: a strand variant region and a heavy chain variant region of SEQ ID NO: 19; a light chain variant region of SEQ ID NO: 7 and a heavy chain variant region of SEQ ID NO: 20; a light chain variant region of SEQ ID NO: 8 and SEQ ID NO: a heavy chain variant region of 21; a light chain variant region of SEQ ID NO: 9 and a heavy chain variant region of SEQ ID NO: 22; a light chain variant region of SEQ ID NO: 10 and a heavy chain of SEQ ID NO: 23. a variant region; a light chain variant region of SEQ ID NO: 11 and a heavy chain variant region of SEQ ID NO: 24; a light chain variant region of SEQ ID NO: 12; and a heavy chain variant region of SEQ ID NO: 25; Is SEQ ID NO: 13 the light chain variable region and SEQ ID NO: 26, a heavy chain variable region. In other specific embodiments, the invention is a one or more isolated nucleic acid molecules encoding a humanized heavy chain and a humanized light chain (which are associated together to form a humanized immunoglobulin having a specific binding to human CD52) Wherein the humanized immunoglobulin binds to an epitope of human CD52 that overlaps with an epitope determined by a mouse monoclonal antibody.

在其他具體實施例,本發明為一種一或更多經分離核酸分子,其編碼人類化重鏈及人類化輕鏈(其在一起會形成具對人類CD52的特定結合的人類化免疫球蛋白),其中該人類化免疫球蛋白結合至包含至少成熟人類CD52的殘基1之抗原決定區;該人類化免疫球蛋白結合至包含至少成熟人類CD52的殘基1、3、4及5之抗原決定區;該人類化免疫球蛋白結合至包含至少成熟人類CD52的殘基1、2、3、4及5之抗原決定區;或是該人類化免疫球蛋白結合至包含至少成熟人類CD52的殘基7、8及9之抗原決定區。在一些具體實施例,該抗原決定區包含至少成熟人類CD52序列的殘基7、8及11。在一些具體實施例,該抗原決定區包含至少成熟人類CD52序列的殘基4及11。In other embodiments, the invention is a one or more isolated nucleic acid molecules encoding a humanized heavy chain and a humanized light chain (which together form a humanized immunoglobulin having a specific binding to human CD52) Wherein the humanized immunoglobulin binds to an epitope comprising residue 1 of at least mature human CD52; the humanized immunoglobulin binds to an antigen comprising residues 1, 3, 4 and 5 of at least mature human CD52 a humanized immunoglobulin that binds to an epitope comprising residues 1, 2, 3, 4, and 5 of at least mature human CD52; or the humanized immunoglobulin binds to a residue comprising at least mature human CD52 The epitopes of 7, 8 and 9. In some embodiments, the epitope comprises at least residues 7, 8 and 11 of the mature human CD52 sequence. In some embodiments, the epitope comprises at least residues 4 and 11 of the mature human CD52 sequence.

在其他具體實施例,本發明為一種一或更多經分離核酸分子,其編碼人類化重鏈及人類化輕鏈(其在一起會形成具對人類CD52的特定結合的人類化免疫球蛋白),其中該人類化免疫球蛋白包含一種輕鏈,其包含由SEQ ID NO: 115、SEQ ID NO: 118、及SEQ ID NO: 121所組成族群選出的一或更多CDR(例如,所有三個該CDR),及/或一種重鏈,其包含由SEQ ID NO: 124、SEQ ID NO: 127、及SEQ ID NO: 130所組成族群選出的一或更多CDR(例如,所有三個該CDR);一種輕鏈,其包含由SEQ ID NO: 116、SEQ ID NO: 119、及SEQ ID NO: 122所組成族群選出的一或更多CDR(例如,所有三個該CDR),及/或一種重鏈,其包含由SEQ ID NO: 125、SEQ ID NO: 128、及SEQ ID NO: 131所組成族群選出的一或更多CDR(例如,所有三個該CDRs);或一種輕鏈,其包含由SEQ ID NO: 117、SEQ ID NO: 120、及SEQ ID NO: 123所組成族群選出的一或更多CDR(例如,所有三個該CDR),及/或一種重鏈,其包含由SEQ ID NO: 126、SEQ ID NO: 129、及SEQ ID NO: 132所組成族群選出的一或更多CDR(例如,所有三個該CDR)。In other embodiments, the invention is a one or more isolated nucleic acid molecules encoding a humanized heavy chain and a humanized light chain (which together form a humanized immunoglobulin having a specific binding to human CD52) Wherein the humanized immunoglobulin comprises a light chain comprising one or more CDRs selected from the group consisting of SEQ ID NO: 115, SEQ ID NO: 118, and SEQ ID NO: 121 ( eg , all three The CDR), and/or a heavy chain comprising one or more CDRs selected from the group consisting of SEQ ID NO: 124, SEQ ID NO: 127, and SEQ ID NO: 130 ( eg , all three of the CDRs) a light chain comprising one or more CDRs selected from the group consisting of SEQ ID NO: 116, SEQ ID NO: 119, and SEQ ID NO: 122 ( eg , all three of the CDRs), and/or A heavy chain comprising one or more CDRs selected from the group consisting of SEQ ID NO: 125, SEQ ID NO: 128, and SEQ ID NO: 131 ( eg , all three of the CDRs); or a light chain, comprising the SEQ ID NO: 117, SEQ ID NO: 120, and SEQ ID NO: 123 Suo one or more CDR selected from the group consisting of (e.g., all three CDR), and / or one heavy chain comprising a SEQ ID NO: 126, SEQ ID NO: 129, and SEQ ID NO: 132 Suo one or more CDR selected from the group consisting of (e.g., all the three CDR) .

在特定具體實施例,本發明為一種一或更多經分離核酸分子,其編碼人類化重鏈及人類化輕鏈(其在一起會形成具對人類CD52的特定結合的人類化免疫球蛋白),其中該人類化免疫球蛋白包含一種輕鏈,其包含SEQ ID NO: 115、SEQ ID NO: 118及SEQ ID NO: 121的CDR及一種重鏈,其包含SEQ ID NO: 124、SEQ ID NO: 127及SEQ ID NO: 130的CDR;一種輕鏈,其包含SEQ ID NO: 116、SEQ ID NO: 119及SEQ ID NO: 122的CDR及一種重鏈,其包含SEQ ID NO: 125、SEQ ID NO: 128及SEQ ID NO: 131的CDR;或一種輕鏈,其包含SEQ ID NO: 117、SEQ ID NO: 120及SEQ ID NO: 123的CDR及一種重鏈,其包含SEQ ID NO: 126、SEQ ID NO:129及SEQ ID NO:132的CDR。In a specific embodiment, the invention is a one or more isolated nucleic acid molecules encoding a humanized heavy chain and a humanized light chain (which together form a humanized immunoglobulin having a specific binding to human CD52) Wherein the humanized immunoglobulin comprises a light chain comprising the CDRs of SEQ ID NO: 115, SEQ ID NO: 118 and SEQ ID NO: 121 and a heavy chain comprising SEQ ID NO: 124, SEQ ID NO CDRs of 127 and SEQ ID NO: 130; a light chain comprising the CDRs of SEQ ID NO: 116, SEQ ID NO: 119 and SEQ ID NO: 122 and a heavy chain comprising SEQ ID NO: 125, SEQ ID NO: 128 and the CDR of SEQ ID NO: 131; or a light chain comprising the CDRs of SEQ ID NO: 117, SEQ ID NO: 120 and SEQ ID NO: 123 and a heavy chain comprising SEQ ID NO: 126. CDRs of SEQ ID NO: 129 and SEQ ID NO: 132.

本發明的一或更多核酸不編碼人類化免疫球蛋白CampathOne or more nucleic acids of the invention do not encode a humanized immunoglobulin Campath .

在其他具體實施例,本發明為一或更多經分離核酸分子,其編碼人類化重鏈及人類化輕鏈(其在一起會形成具對人類CD52的特定結合的人類化免疫球蛋白),其中該人類化免疫球蛋白對於醣化人類CD52較對於非-醣化或去-醣化人類CD52具有更大結合親和力,例如,顯現對醣化人類CD52特定的結合。人類化免疫球蛋白可結合至包含其N-鍵結碳水化合物基團的成熟人類CD52上的抗原決定區。此抗原決定區亦可包含至少成熟人類CD52序列的殘基1,至少成熟人類CD52序列的殘基3,至少成熟人類CD52序列的殘基1、3、4及5,或是至少成熟人類CD52序列的殘基1、2、3、4及5。In other specific embodiments, the invention is one or more isolated nucleic acid molecules encoding a humanized heavy chain and a humanized light chain (which together form a humanized immunoglobulin having a specific binding to human CD52), Wherein the humanized immunoglobulin has greater binding affinity for glycosylated human CD52 than for non-glycated or de-glycosylated human CD52, for example, exhibiting specific binding to glycosylated human CD52. The humanized immunoglobulin can bind to an epitope on mature human CD52 comprising its N -bonded carbohydrate group. The epitope may also comprise at least residue 1 of the mature human CD52 sequence, at least residue 3 of the mature human CD52 sequence, at least residues 1, 3, 4 and 5 of the mature human CD52 sequence, or at least the mature human CD52 sequence. Residues 1, 2, 3, 4 and 5.

在其他具體實施例,本發明為一種經分離核酸分子,其編碼人類化輕鏈,其包含SEQ ID NO:3、SEQ ID NO:4、SEQ ID NO:5、SEQ ID NO:6、SEQ ID NO:7、SEQ ID NO:8、SEQ ID NO:9、SEQ ID NO:10、SEQ ID NO:11、SEQ ID NO:12或SEQ ID NO:13的一或更多CDR(例如有三個該CDR),其中該人類化輕鏈不為Campath的人類化輕鏈。In other specific embodiments, the invention is an isolated nucleic acid molecule encoding a humanized light chain comprising SEQ ID NO:3, SEQ ID NO:4, SEQ ID NO:5, SEQ ID NO:6, SEQ ID NO: 7, SEQ ID NO: 8, SEQ ID NO: 9, SEQ ID NO: 10, SEQ ID NO: 11, SEQ ID NO: 12 or SEQ ID NO: one or more CDR 13 (e.g., the three The CDR), wherein the humanized light chain is not Campath Humanized light chain.

在其他具體實施例,本發明為一種經分離核酸分子,其編碼人類化重鏈,其包含SEQ ID NO:16、SEQ ID NO:17、SEQ ID NO:18、SEQ ID NO:19、SEQ ID NO:20、SEQ ID NO:21、SEQ ID NO:22、SEQ ID NO:23、SEQ ID NO:24、SEQ ID NO:25、SEQ ID NO:26、或SEQ ID NO:137的一或更多CDR(例如,所有三個該CDR),其中該人類化重鏈不為Campath的人類化重鏈。In other specific embodiments, the invention is an isolated nucleic acid molecule encoding a humanized heavy chain comprising SEQ ID NO: 16, SEQ ID NO: 17, SEQ ID NO: 18, SEQ ID NO: 19, SEQ ID One or more of NO: 20, SEQ ID NO: 21, SEQ ID NO: 22, SEQ ID NO: 23, SEQ ID NO: 24, SEQ ID NO: 25, SEQ ID NO: 26, or SEQ ID NO: Multiple CDRs ( eg, all three of the CDRs), wherein the humanized heavy chain is not Campath Humanized heavy chain.

在其他具體實施例,本發明為一種經分離核酸分子,其編碼人類化輕鏈,其包含由SEQ ID NO:27、SEQ ID NO:28、SEQ ID NO:29、SEQ ID NO:30、SEQ ID NO:31、SEQ ID NO:32、SEQ ID NO:33、SEQ ID NO:34、SEQ ID NO:35、SEQ ID NO:36、SEQ ID NO:37、SEQ ID NO:38、SEQ ID NO:39、SEQ ID NO:40、SEQ ID NO:41、SEQ ID NO:42、SEQ ID NO:43、SEQ ID NO:44、SEQ ID NO:45、SEQ ID NO:46、SEQ ID NO:47、及SEQ ID NO:48或是其組合所組成族群選出的一或更多CDR,其中該人類化輕鏈不為Campath的人類化輕鏈。In other specific embodiments, the invention is an isolated nucleic acid molecule encoding a humanized light chain comprising SEQ ID NO:27, SEQ ID NO:28, SEQ ID NO:29, SEQ ID NO:30, SEQ ID NO: 31, SEQ ID NO: 32, SEQ ID NO: 33, SEQ ID NO: 34, SEQ ID NO: 35, SEQ ID NO: 36, SEQ ID NO: 37, SEQ ID NO: 38, SEQ ID NO 39, SEQ ID NO: 40, SEQ ID NO: 41, SEQ ID NO: 42, SEQ ID NO: 43, SEQ ID NO: 44, SEQ ID NO: 45, SEQ ID NO: 46, SEQ ID NO: 47 And one or more CDRs selected from the group consisting of SEQ ID NO: 48 or a combination thereof, wherein the humanized light chain is not Campath Humanized light chain.

在其他具體實施例,本發明為一種經分離核酸分子,其編碼人類化重鏈,其包含由SEQ ID NO:49、SEQ ID NO:50、SEQ ID NO:51、SEQ ID NO:52、SEQ ID NO:53、SEQ ID NO:54、SEQ ID NO:55、SEQ ID NO:56、SEQ ID NO:57、SEQ ID NO:58、SEQ ID NO:59、SEQ ID NO:60、SEQ ID NO:61、SEQ ID NO:62、SEQ ID NO:63、SEQ ID NO:64、SEQ ID NO:65、SEQ ID NO:66、SEQ ID NO:67、SEQ ID NO:68、SEQ ID NO:69、SEQ ID NO:70、SEQ ID NO:71、SEQ ID NO:72、SEQ ID NO:73、SEQ ID NO:74、及SEQ ID NO:294或是其組合所組成族群選出的一或更多CDR,其中該人類化重鏈不為Campath的人類化重鏈。In other specific embodiments, the invention is an isolated nucleic acid molecule encoding a humanized heavy chain comprising SEQ ID NO: 49, SEQ ID NO: 50, SEQ ID NO: 51, SEQ ID NO: 52, SEQ ID NO: 53, SEQ ID NO: 54, SEQ ID NO: 55, SEQ ID NO: 56, SEQ ID NO: 57, SEQ ID NO: 58, SEQ ID NO: 59, SEQ ID NO: 60, SEQ ID NO :61, SEQ ID NO: 62, SEQ ID NO: 63, SEQ ID NO: 64, SEQ ID NO: 65, SEQ ID NO: 66, SEQ ID NO: 67, SEQ ID NO: 68, SEQ ID NO: 69 One or more selected from the group consisting of SEQ ID NO: 70, SEQ ID NO: 71, SEQ ID NO: 72, SEQ ID NO: 73, SEQ ID NO: 74, and SEQ ID NO: 294, or a combination thereof CDR, wherein the humanized heavy chain is not Campath Humanized heavy chain.

在其他具體實施例,本發明為一種經分離核酸分子,其編碼人類化輕鏈,其包含由SEQ ID NO: 115、SEQ ID NO: 118、及SEQ ID NO: 121所組成族群選出的一或更多CDR(例如,所有三個該CDR);一種人類化輕鏈,其包含由SEQ ID NO: 116、SEQ ID NO: 119、及SEQ ID NO: 122所組成族群選出的一或更多CDR(例如,所有三個該CDR);或是一種人類化輕鏈,其包含由SEQ ID NO: 117、SEQ ID NO: 120、及SEQ ID NO: 123所組成族群選出的一或更多CDR(例如,所有三個該CDR)。In other specific embodiments, the invention is an isolated nucleic acid molecule encoding a humanized light chain comprising one selected from the group consisting of SEQ ID NO: 115, SEQ ID NO: 118, and SEQ ID NO: 121 More CDRs ( eg, all three of the CDRs); a humanized light chain comprising one or more CDRs selected from the group consisting of SEQ ID NO: 116, SEQ ID NO: 119, and SEQ ID NO: 122 ( eg, all three of the CDRs); or a humanized light chain comprising one or more CDRs selected from the group consisting of SEQ ID NO: 117, SEQ ID NO: 120, and SEQ ID NO: 123 ( For example, all three of the CDRs).

在其他具體實施例,本發明為一種經分離核酸分子,其編碼人類化重鏈,其包含由SEQ ID NO: 124、SEQ ID NO: 127、及SEQ ID NO: 130所組成族群選出的一或更多CDR(例如,所有三個該CDR);人類化重鏈,其包含由SEQ ID NO: 125、SEQ ID NO: 128、及SEQ ID NO: 131所組成族群選出的一或更多CDR(例如,所有三個該CDR);或是人類化重鏈,其包含由SEQ ID NO: 126、SEQ ID NO: 129、及SEQ ID NO: 132所組成族群選出的一或更多CDR(例如,所有三個該CDR)。In other specific embodiments, the invention is an isolated nucleic acid molecule encoding a humanized heavy chain comprising one selected from the group consisting of SEQ ID NO: 124, SEQ ID NO: 127, and SEQ ID NO: 130 More CDRs ( eg, all three of the CDRs); a humanized heavy chain comprising one or more CDRs selected from the group consisting of SEQ ID NO: 125, SEQ ID NO: 128, and SEQ ID NO: 131 For example, all three of the CDRs; or a humanized heavy chain comprising one or more CDRs selected from the group consisting of SEQ ID NO: 126, SEQ ID NO: 129, and SEQ ID NO: 132 ( eg, All three of the CDRs).

本發明亦相關於一種重組載體(例如,表現載體,其包含哺乳動物細胞表現載體),其包含編碼本發明人類化免疫球蛋白(例如,人類化輕鏈及人類化重鏈)、人類化輕鏈、或人類化重鏈的核酸。在一些具體實施例,本發明為一種重組載體,其包含編碼人類化免疫球蛋白的核酸,人類化免疫球蛋白包含含有SEQ ID NO:3的一或更多CDR(例如,所有三個CDR)的輕鏈及含有SEQ ID NO:16的一或更多CDR(例如,所有三個CDR)的重鏈;含有SEQ ID NO:4的一或更多CDR(例如,所有三個CDR)的輕鏈及含有SEQ ID NO:17的一或更多CDR(例如,所有三個CDR)的重鏈;含有SEQ ID NO:5的一或更多CDR(例如,所有三個CDR)的輕鏈及含有SEQ ID NO:18的一或更多CDR(例如,所有三個CDR)的重鏈;含有SEQ ID NO:6的一或更多CDR(例如,所有三個CDR)的輕鏈及含有SEQ ID NO:19的一或更多CDR(例如,所有三個CDR)的重鏈;含有SEQ ID NO:7的一或更多CDR(例如,所有三個CDR)的輕鏈及含有SEQ ID NO:20的一或更多CDR(例如,所有三個CDR)的重鏈;含有SEQ ID NO:8的一或更多CDR(例如,所有三個CDR)的輕鏈及含有SEQ ID NO:21的一或更多CDR(例如,所有三個CDR)的重鏈;含有SEQ ID NO:9的一或更多CDR(例如,所有三個CDR)的輕鏈及含有SEQ ID NO:22的一或更多CDR(例如,所有三個CDR)的重鏈;含有SEQ ID NO:10的一或更多CDR(例如,所有三個CDR)的輕鏈及含有SEQ ID NO:23的一或更多CDR(例如,所有三個CDR)的重鏈;含有SEQ ID NO:11的一或更多CDR(例如,所有三個CDR)的輕鏈及含有SEQ ID NO:24的一或更多CDR(例如,所有三個CDR)的重鏈;含有SEQ ID NO:12的一或更多CDR(例如,所有三個CDR)的輕鏈及含有SEQ ID NO:25的一或更多CDR(例如,所有三個CDR)的重鏈;含有SEQID NO: 12的一或更多CDR(例如,所有三個CDR)的輕鏈及含有SEQ ID NO:137的一或更多CDR(例如,所有三個CDR)的重鏈;或是含有SEQ ID NO:13的一或更多CDR(例如,所有三個CDR)的輕鏈及含有SEQ ID NO:26的一或更多CDR(例如,所有三個CDR)的重鏈。The invention also relates to a recombinant vector ( eg, a expression vector comprising a mammalian cell expression vector) comprising a humanized immunoglobulin encoding the invention (eg, a humanized light chain and a humanized heavy chain), which is lightly humanized A nucleic acid that is a chain, or a humanized heavy chain. In some embodiments, the invention is a recombinant vector comprising a nucleic acid encoding a humanized immunoglobulin comprising one or more CDRs comprising SEQ ID NO: 3 ( eg , all three CDRs) Light chain and heavy chain comprising one or more CDRs of SEQ ID NO: 16 ( eg , all three CDRs); light comprising one or more CDRs of SEQ ID NO: 4 ( eg , all three CDRs) a heavy chain comprising a strand and one or more CDRs comprising SEQ ID NO: 17 ( eg , all three CDRs); a light chain comprising one or more CDRs of SEQ ID NO: 5 ( eg , all three CDRs) a heavy chain comprising one or more CDRs of SEQ ID NO: 18 ( eg , all three CDRs); a light chain comprising one or more CDRs of SEQ ID NO: 6 ( eg , all three CDRs) and comprising SEQ ID NO: heavy chain of one or more CDRs ( eg , all three CDRs) of 19; light chain comprising one or more CDRs of SEQ ID NO: 7 ( eg , all three CDRs) and comprising SEQ ID NO : one or more of the CDRs of 20 (e.g., all three CDR) of a heavy chain; comprising SEQ ID NO: CDRs of one or more (e.g., all three CDR). 8 and a light chain comprising SEQ ID NO: 21 is CDRs of one or more (e.g., the Three CDR) of a heavy chain; comprising SEQ ID NO: CDR 9 one or more (e.g., all three CDR) and a light chain comprising SEQ ID NO: one or more CDR 22 (e.g., all three Heavy chain of CDR); light chain comprising one or more CDRs of SEQ ID NO: 10 ( eg , all three CDRs) and one or more CDRs comprising SEQ ID NO: 23 ( eg , all three CDRs) Heavy chain; light chain comprising one or more CDRs of SEQ ID NO: 11 ( eg , all three CDRs) and one or more CDRs comprising SEQ ID NO: 24 ( eg , all three CDRs) a chain; a light chain comprising one or more CDRs of SEQ ID NO: 12 ( eg , all three CDRs) and a heavy chain comprising one or more CDRs of SEQ ID NO: 25 ( eg , all three CDRs); a light chain comprising one or more CDRs of SEQ ID NO: 12 ( eg, all three CDRs) and a heavy chain comprising one or more CDRs of SEQ ID NO: 137 ( eg, all three CDRs); or The light chain of one or more CDRs ( eg, all three CDRs) of SEQ ID NO: 13 and the heavy chain comprising one or more CDRs of SEQ ID NO: 26 ( eg, all three CDRs).

在其他具體實施例,重組載體包含編碼人類化輕鏈的核酸,其中該人類化輕鏈包含由SEQ ID NO:27、SEQ ID NO:28、SEQ ID NO:29、SEQ ID NO:30、SEQ ID NO:31、SEQ ID NO:32、SEQ ID NO:33、SEQ ID NO:34、SEQ ID NO:35、SEQ ID NO:36、SEQ ID NO:37、SEQ ID NO:38、SEQ ID NO:39、SEQ ID NO:40、SEQ ID NO:41、SEQ ID NO:42、SEQ ID NO:43、SEQ ID NO:44、SEQ ID NO:45、SEQ ID NO:46、SEQ ID NO:47、及SEQ ID NO:48或是其組合所組成族群選出的一或更多CDR,其中該人類化輕鏈不為Campath的人類化輕鏈。In other specific embodiments, the recombinant vector comprises a nucleic acid encoding a humanized light chain, wherein the humanized light chain comprises SEQ ID NO:27, SEQ ID NO:28, SEQ ID NO:29, SEQ ID NO:30, SEQ ID NO: 31, SEQ ID NO: 32, SEQ ID NO: 33, SEQ ID NO: 34, SEQ ID NO: 35, SEQ ID NO: 36, SEQ ID NO: 37, SEQ ID NO: 38, SEQ ID NO 39, SEQ ID NO: 40, SEQ ID NO: 41, SEQ ID NO: 42, SEQ ID NO: 43, SEQ ID NO: 44, SEQ ID NO: 45, SEQ ID NO: 46, SEQ ID NO: 47 And one or more CDRs selected from the group consisting of SEQ ID NO: 48 or a combination thereof, wherein the humanized light chain is not Campath Humanized light chain.

在其他具體實施例,重組載體包含編碼人類化重鏈的核酸,其中該人類化重鏈包含由SEQ ID NO:49、SEQ ID NO:50、SEQ ID NO:51、SEQ ID NO:52、SEQ ID NO:53、SEQ ID NO:54、SEQ ID NO:55、SEQ ID NO:56、SEQ ID NO:57、SEQ ID NO:58、SEQ ID NO:59、SEQ ID NO:60、SEQ ID NO:61、SEQ ID NO:62、SEQ ID NO:63、SEQ ID NO:64、SEQ ID NO:65、SEQ ID NO:66、SEQ ID NO:67、SEQ ID NO:68、SEQ ID NO:69、SEQ ID NO:70、SEQ ID NO:71、SEQ ID NO:72、SEQ ID NO:73、SEQ ID NO:74、及SEQ ID NO: 294或是其組合所組成族群選出的一或更多CDR,其中該人類化重鏈不為Campath的人類化重鏈。In other specific embodiments, the recombinant vector comprises a nucleic acid encoding a humanized heavy chain, wherein the humanized heavy chain comprises SEQ ID NO: 49, SEQ ID NO: 50, SEQ ID NO: 51, SEQ ID NO: 52, SEQ ID NO: 53, SEQ ID NO: 54, SEQ ID NO: 55, SEQ ID NO: 56, SEQ ID NO: 57, SEQ ID NO: 58, SEQ ID NO: 59, SEQ ID NO: 60, SEQ ID NO :61, SEQ ID NO: 62, SEQ ID NO: 63, SEQ ID NO: 64, SEQ ID NO: 65, SEQ ID NO: 66, SEQ ID NO: 67, SEQ ID NO: 68, SEQ ID NO: 69 One or more selected from the group consisting of SEQ ID NO: 70, SEQ ID NO: 71, SEQ ID NO: 72, SEQ ID NO: 73, SEQ ID NO: 74, and SEQ ID NO: 294, or a combination thereof CDR, wherein the humanized heavy chain is not Campath Humanized heavy chain.

在一些具體實施例,本發明提供包含一個核酸分子的一個重組載體,或是包含編碼人類化重鏈及人類化輕鏈(其在一起會形成具對人類CD52的特定結合的人類化免疫球蛋白)核酸分子的一對重組載體,,其中該人類化免疫球蛋白結合至與老鼠單株抗體相同的位於人類CD52之抗原決定區,其中該老鼠單株抗體包含SEQ ID NO: 3的輕鏈變異區及SEQ ID NO: 16的重鏈變異區;SEQ ID NO: 4的輕鏈變異區及SEQ ID NO: 17的重鏈變異區;SEQ ID NO: 5的輕鏈變異區及SEQ ID NO: 18的重鏈變異區;SEQ ID NO: 6的輕鏈變異區及SEQ ID NO: 19的重鏈變異區;SEQ ID NO: 7的輕鏈變異區及SEQ ID NO: 20的重鏈變異區;SEQ ID NO: 8的輕鏈變異區及SEQ ID NO: 21的重鏈變異區;SEQ ID NO: 9的輕鏈變異區及SEQ ID NO: 22的重鏈變異區;SEQ ID NO: 10的輕鏈變異區及SEQ ID NO: 23的重鏈變異區;SEQ ID NO: 11的輕鏈變異區及SEQ ID NO: 24的重鏈變異區;SEQ ID NO: 12的輕鏈變異區及SEQ ID NO: 25的重鏈變異區;或是SEQ ID NO: 13的輕鏈變異區及SEQ ID NO: 26的重鏈變異區。在其他具體實施例,本發明提供包含一個核酸分子的一個重組載體,或是包含編碼人類化重鏈及人類化輕鏈(其在一起會形成具對人類CD52的特定結合的人類化免疫球蛋白)核酸分子的一對重組載體,其中該人類化免疫球蛋白結合至於人類CD52上的抗原決定區,此抗原決定區與老鼠單株抗體所結合的抗原決定區重疊。In some embodiments, the invention provides a recombinant vector comprising a nucleic acid molecule, or a humanized immunoglobulin comprising a humanized heavy chain and a humanized light chain that together form a specific binding to human CD52 a pair of recombinant vectors of a nucleic acid molecule, wherein the humanized immunoglobulin binds to an epitope of human CD52 identical to a mouse monoclonal antibody, wherein the mouse monoclonal antibody comprises a light chain variant of SEQ ID NO: a region and a heavy chain variant region of SEQ ID NO: 16; a light chain variant region of SEQ ID NO: 4 and a heavy chain variant region of SEQ ID NO: 17; a light chain variant region of SEQ ID NO: 5 and SEQ ID NO: a heavy chain variant region of 18; a light chain variant region of SEQ ID NO: 6 and a heavy chain variant region of SEQ ID NO: 19; a light chain variant region of SEQ ID NO: 7 and a heavy chain variant region of SEQ ID NO: ; the light chain variant region of SEQ ID NO: 8 and the heavy chain variant region of SEQ ID NO: 21; the light chain variant region of SEQ ID NO: 9 and the heavy chain variant region of SEQ ID NO: 22; SEQ ID NO: 10 Light chain variant region and heavy chain variant region of SEQ ID NO: 23; light chain variant region of SEQ ID NO: 11 and heavy chain variant of SEQ ID NO: Region; SEQ ID NO: 12 and a light chain variable region and SEQ ID NO: 25, a heavy chain variable region; or SEQ ID NO: 13 the light chain variable region and SEQ ID NO: 26, a heavy chain variable region. In other embodiments, the invention provides a recombinant vector comprising a nucleic acid molecule, or a humanized immunoglobulin comprising a humanized heavy chain and a humanized light chain that together form a specific binding to human CD52 A pair of recombinant vectors of nucleic acid molecules, wherein the humanized immunoglobulin binds to an epitope of human CD52 that overlaps with an epitope determined by a mouse monoclonal antibody.

在其他具體實施例,該重組載體包含一個核酸分子,或是一對包含編碼人類化重鏈及人類化輕鏈(其在一起會形成具對人類CD52的特定結合的人類化免疫球蛋白)核酸分子的重組載體,其中該人類化免疫球蛋白結合至包含至少成熟人類CD52的殘基1之抗原決定區;結合至包含至少成熟人類CD52的殘基1、3、4及5之抗原決定區;結合至包含至少成熟人類CD52的殘基1、2、3、4及5之抗原決定區;或是結合至包含至少成熟人類CD52的殘基7、8及9之抗原決定區。在一些具體實施例,該抗原決定區包含至少成熟人類CD52序列的殘基7、8及11。在一些具體實施例,該抗原決定區包含至少成熟人類CD52序列的殘基4及11。In other embodiments, the recombinant vector comprises a nucleic acid molecule, or a pair of nucleic acids comprising a humanized heavy chain and a humanized light chain that together form a humanized immunoglobulin having a specific binding to human CD52. a recombinant vector of a molecule, wherein the humanized immunoglobulin binds to an epitope comprising residue 1 of at least mature human CD52; binds to an epitope comprising residues 1, 3, 4 and 5 of at least mature human CD52; Binding to an epitope comprising residues 1, 2, 3, 4 and 5 of at least mature human CD52; or binding to an epitope comprising residues 7, 8 and 9 of at least mature human CD52. In some embodiments, the epitope comprises at least residues 7, 8 and 11 of the mature human CD52 sequence. In some embodiments, the epitope comprises at least residues 4 and 11 of the mature human CD52 sequence.

在一些具體實施例,該重組載體包含一個核酸分子,或是一對包含編碼人類化重鏈及人類化輕鏈(其在一起會形成具對人類CD52的特定結合的人類化免疫球蛋白)核酸分子的重組載體,其中該人類化免疫球蛋白包含含有由SEQ ID NO: 115、SEQ ID NO: 118、及SEQ ID NO: 121所組成族群選出的一或更多CDR(例如,所有三個該CDR)之一種輕鏈,及/或包含由SEQ ID NO: 124、SEQ ID NO: 127、及SEQ ID NO: 130所組成族群選出的一或更多CDR(例如,所有三個該CDR)的一種重鏈;包含由SEQ ID NO: 116、SEQ ID NO: 119、及SEQ ID NO: 122所組成族群選出的一或更多CDR(例如,所有三個該CDR)的一種輕鏈,及/或包含由SEQ ID NO: 125、SEQ ID NO: 128、及SEQ ID NO: 131所組成族群選出的一或更多CDR(例如,所有三個該CDR)的一種重鏈;或包含由SEQ ID NO: 117、SEQ ID NO: 120、及SEQ ID NO: 123所組成族群選出的一或更多CDR(例如,所有三個該CDR)的一種輕鏈,及/或包含由SEQ ID NO: 126、SEQ ID NO: 129、及SEQ ID NO: 132所組成族群選出的一或更多CDR(例如,所有三個該CDR)的一種重鏈。In some embodiments, the recombinant vector comprises a nucleic acid molecule, or a pair of nucleic acids comprising a humanized heavy chain and a humanized light chain that together form a humanized immunoglobulin having a specific binding to human CD52. A recombinant vector of a molecule, wherein the humanized immunoglobulin comprises one or more CDRs selected from the group consisting of SEQ ID NO: 115, SEQ ID NO: 118, and SEQ ID NO: 121 ( eg, all three of a light chain of CDR), and/or comprising one or more CDRs selected from the group consisting of SEQ ID NO: 124, SEQ ID NO: 127, and SEQ ID NO: 130 ( eg, all three of the CDRs) A heavy chain; a light chain comprising one or more CDRs selected from the group consisting of SEQ ID NO: 116, SEQ ID NO: 119, and SEQ ID NO: 122 ( eg , all three of the CDRs), and/ Or a heavy chain comprising one or more CDRs selected from the group consisting of SEQ ID NO: 125, SEQ ID NO: 128, and SEQ ID NO: 131 ( eg , all three of the CDRs); or comprising SEQ ID NO: 117, SEQ ID NO: 120, and SEQ ID NO: 123 Suo one or more CDR selected from the group consisting of (e.g., all three CDR) a light chain, and / or encompassed by SEQ ID NO: 126, SEQ ID NO: 129, and SEQ ID NO: one or more CDR selected from the group consisting of 132 (e.g., all three of the CDR), A heavy chain.

在某些具體實施例,該重組載體包含一個核酸分子,或是一對包含編碼人類化重鏈及人類化輕鏈(其在一起會形成具對人類CD52的特定結合的人類化免疫球蛋白)核酸分子的重組載體,其中該人類化免疫球蛋白包含含有SEQ ID NO: 115、SEQ ID NO: 118及SEQ ID NO: 121的CDR之輕鏈及包含SEQ ID NO: 124、SEQ ID NO: 127及SEQ ID NO: 130的CDR之重鏈;包含SEQ ID NO: 116、SEQ ID NO: 119及SEQ ID NO: 122的CDR之輕鏈及包含SEQ ID NO: 125、SEQ ID NO: 128及SEQ ID NO: 131的CDR之重鏈;或包含SEQ ID NO: 117、SEQ ID NO: 120及SEQ ID NO: 123的CDR之輕鏈及包含SEQ ID NO: 126、SEQ ID NO: 129及SEQ ID NO: 132的CDR之重鏈。In certain embodiments, the recombinant vector comprises a nucleic acid molecule, or a pair comprising a humanized heavy chain and a humanized light chain (which together form a humanized immunoglobulin having a specific binding to human CD52) A recombinant vector of a nucleic acid molecule, wherein the humanized immunoglobulin comprises a light chain comprising the CDRs of SEQ ID NO: 115, SEQ ID NO: 118 and SEQ ID NO: 121 and comprises SEQ ID NO: 124, SEQ ID NO: 127 And a heavy chain of the CDR of SEQ ID NO: 130; a light chain comprising the CDRs of SEQ ID NO: 116, SEQ ID NO: 119 and SEQ ID NO: 122 and comprising SEQ ID NO: 125, SEQ ID NO: 128 and SEQ ID NO: the heavy chain of the CDR of 131; or the light chain comprising the CDRs of SEQ ID NO: 117, SEQ ID NO: 120 and SEQ ID NO: 123 and comprising SEQ ID NO: 126, SEQ ID NO: 129 and SEQ ID NO: The heavy chain of the CDR of 132.

在本發明重組載體或數個載體中的一或更多核酸不編碼人類化免疫球蛋白CampathOne or more nucleic acids in a recombinant vector or vectors of the invention do not encode a humanized immunoglobulin Campath .

在其他具體實施例,該重組載體包含一個核酸分子,或是一對編碼人類化重鏈及人類化輕鏈(其關聯在一起而形成具對人類CD52的特定結合的人類化免疫球蛋白核酸分子的重組載體,其中該人類化免疫球蛋白對於醣化人類CD52較對於非-醣化或去-醣化人類CD52具有更大結合親和力,例如,顯現對於醣化人類CD52特定的結合。人類化免疫球蛋白可結合至包含其N-鍵結碳水化合物基團的成熟人類CD52上的抗原決定區。此抗原決定區亦可包含至少成熟人類CD52序列的殘基1,至少成熟人類CD52序列的殘基3,至少成熟人類CD52序列的殘基1、3、4及5,或是至少成熟人類CD52序列的殘基1、2、3、4及5。In other embodiments, the recombinant vector comprises a nucleic acid molecule, or a pair of humanized heavy chains and humanized light chains that are associated to form a humanized immunoglobulin nucleic acid molecule having a specific binding to human CD52. A recombinant vector, wherein the humanized immunoglobulin has greater binding affinity for glycosylated human CD52 than for non-glycated or de-glycosylated human CD52, for example, exhibiting specific binding to glycosylated human CD52. Humanized immunoglobulin can bind To an epitope on mature human CD52 comprising its N -bonded carbohydrate group. The epitope may also comprise at least residue 1 of the mature human CD52 sequence, at least residue 3 of the mature human CD52 sequence, at least mature Residues 1, 3, 4, and 5 of the human CD52 sequence, or at least residues 1, 2, 3, 4, and 5 of the mature human CD52 sequence.

在其他具體實施例,該重組載體包含一個核酸分子,其編碼人類化輕鏈,其包含SEQ ID NO:3、SEQ ID NO:4、SEQ ID NO:5、SEQ ID NO:6、SEQ ID NO:7、SEQ ID NO:8、SEQ ID NO:9、SEQ ID NO:10、SEQ ID NO:11、SEQ ID NO:12或SEQ ID NO:13的一或更多CDR(例如,所有三個該CDRs),其中該人類化輕鏈不為Campath的人類化輕鏈。In other specific embodiments, the recombinant vector comprises a nucleic acid molecule encoding a humanized light chain comprising SEQ ID NO:3, SEQ ID NO:4, SEQ ID NO:5, SEQ ID NO:6, SEQ ID NO : 7, one or more CDRs of SEQ ID NO: 8, SEQ ID NO: 9, SEQ ID NO: 10, SEQ ID NO: 11, SEQ ID NO: 12 or SEQ ID NO: 13 ( eg , all three The CDRs), wherein the humanized light chain is not for Campath Humanized light chain.

在其他具體實施例,該重組載體包含一個核酸分子,其編碼人類化重鏈,其包含SEQ ID NO: 16、SEQ ID NO:17、SEQ ID NO:18、SEQ ID NO:19、SEQ ID NO:20、SEQ ID NO:21、SEQ ID NO:22、SEQ ID NO:23、SEQ ID NO:24、SEQ ID NO:25、SEQ ID NO:26、或SEQ ID NO:137的一或更多CDR(例如,所有三個該CDR),其中該人類化重鏈不為Campath的人類化重鏈。In other specific embodiments, the recombinant vector comprises a nucleic acid molecule encoding a humanized heavy chain comprising SEQ ID NO: 16, SEQ ID NO: 17, SEQ ID NO: 18, SEQ ID NO: 19, SEQ ID NO :20, one or more of SEQ ID NO: 21, SEQ ID NO: 22, SEQ ID NO: 23, SEQ ID NO: 24, SEQ ID NO: 25, SEQ ID NO: 26, or SEQ ID NO: 137 CDRs ( eg , all three of the CDRs), wherein the humanized heavy chain is not Campath Humanized heavy chain.

在其他具體實施例,該重組載體包含一個核酸分子,其編碼人類化輕鏈,其包含由SEQ ID NO: 115、SEQ ID NO: 118、及SEQ ID NO: 121所組成族群選出的一或更多CDR(例如,所有三個該CDR);一種人類化輕鏈,其包含由SEQ ID NO: 116、SEQ ID NO: 119、及SEQ ID NO: 122所組成族群選出的一或更多CDR(例如,所有三個該CDR);或是一種人類化輕鏈,其包含由SEQ ID NO: 117、SEQ ID NO: 120、及SEQ ID NO: 123所組成族群選出的一或更多CDR(例如,所有三個該CDR),其中該人類化輕鏈不為Campath的人類化輕鏈。In other specific embodiments, the recombinant vector comprises a nucleic acid molecule encoding a humanized light chain comprising one or more selected from the group consisting of SEQ ID NO: 115, SEQ ID NO: 118, and SEQ ID NO: 121 Multiple CDRs ( eg , all three of the CDRs); a humanized light chain comprising one or more CDRs selected from the group consisting of SEQ ID NO: 116, SEQ ID NO: 119, and SEQ ID NO: 122 For example, all three of the CDRs; or a humanized light chain comprising one or more CDRs selected from the group consisting of SEQ ID NO: 117, SEQ ID NO: 120, and SEQ ID NO: 123 ( eg, , all three of the CDRs), wherein the humanized light chain is not for Campath Humanized light chain.

在其他具體實施例,該重組載體包含一個核酸分子,其編碼包含由SEQ ID NO: 124、SEQ ID NO: 127、及SEQ ID NO: 130所組成族群選出的一或更多CDR(例如,所有三個該CDR)的一種人類化重鏈;包含由SEQ ID NO: 125、SEQ ID NO: 128、及SEQ ID NO: 131所組成族群選出的一或更多CDR(例如,所有三個該CDR)的一種人類化重鏈;包含由SEQ ID NO: 126、SEQ ID NO: 129及SEQ ID NO: 132所組成族群選出的一或更多CDR(例如,所有三個該CDR)的一種人類化重鏈,其中該人類化重鏈不為Campath的人類化重鏈。In other specific embodiments, the recombinant vector comprises a nucleic acid molecule encoding one or more CDRs selected from the group consisting of SEQ ID NO: 124, SEQ ID NO: 127, and SEQ ID NO: 130 ( eg, all a humanized heavy chain of three of said CDRs; comprising one or more CDRs selected from the group consisting of SEQ ID NO: 125, SEQ ID NO: 128, and SEQ ID NO: 131 ( eg, all three of the CDRs) a humanized heavy chain; a humanization comprising one or more CDRs selected from the group consisting of SEQ ID NO: 126, SEQ ID NO: 129, and SEQ ID NO: 132 ( eg, all three of the CDRs) Heavy chain, wherein the humanized heavy chain is not Campath Humanized heavy chain.

在特定具體實施例,本發明重組載體為表現載體,例如哺乳動物細胞表現載體。在某些具體實施例,載體係為一種質粒或是病毒載體(例如,腺病毒或AAV載體)。In a specific embodiment, the recombinant vector of the invention is a performance vector, such as a mammalian cell expression vector. In certain embodiments, the vector is a plasmid or a viral vector ( eg, an adenovirus or an AAV vector).

本發明亦相關於一種包含編碼本發明人類化免疫球蛋白(人類化輕鏈及人類化重鏈)、人類化輕鏈或人類化重鏈的(一或更多)核酸(例如,重組)的宿主細胞。在一些具體實施例,該宿主細胞包含一種本發明重組載體(例如,表現載體,其包含哺乳動物細胞表現載體)。The invention also relates to a (one or more) nucleic acid ( eg, recombinant) comprising a humanized immunoglobulin (humanized light chain and humanized heavy chain), a humanized light chain or a humanized heavy chain of the invention. Host cell. In some embodiments, the host cell comprises a recombinant vector of the invention ( e.g., an expression vector comprising a mammalian cell expression vector).

在特定具體實施例,該宿主細胞包含一種編碼人類化輕鏈或人類化重鏈的核酸(一或更多核酸),其中人類化輕鏈及人類化重鏈在一起會形成具對人類CD52的特定結合的人類化免疫球蛋白及其中該人類化免疫球蛋白包含含有SEQ ID NO:3的一或更多CDR(例如,所有三個CDR)之輕鏈及含有SEQ ID NO:16的一或更多CDR(例如,所有三個CDR)之重鏈;含有SEQ ID NO:4的一或更多CDR(例如,所有三個CDR)之輕鏈及含有SEQ ID NO:17的一或更多CDR(例如,所有三個CDR)之重鏈;含有SEQ ID NO:5的一或更多CDR(例如,所有三個CDR)之輕鏈及含有SEQ ID NO:18的一或更多CDR(例如,所有三個CDR之重鏈;含有SEQ ID NO:6的一或更多CDR(例如,所有三個CDR)之輕鏈及含有SEQ ID NO:19的一或更多CDR(例如,所有三個CDR)之重鏈;含有SEQ ID NO:7的一或更多CDR(例如,所有三個CDR)之輕鏈及含有SEQ ID NO:20的一或更多CDR(例如,所有三個CDR)之重鏈;含有SEQ ID NO:8的一或更多CDR(例如,所有三個CDR)之輕鏈及含有SEQ ID NO:21的一或更多CDR(例如,所有三個CDR)之重鏈;含有SEQ ID NO:9的一或更多CDR(例如,所有三個CDR)之輕鏈及含有SEQ ID NO:22的一或更多CDR(例如,所有三個CDR)之重鏈;含有SEQ ID NO:10的一或更多CDR( ,所有三個CDR)之輕鏈及含有SEQ ID NO:23的一或更多CDR(例如,所有三個CDR)之重鏈;含有SEQ ID NO:11的一或更多CDR(例如,所有三個CDR)之輕鏈及含有SEQ ID NO:24的一或更多CDR(例如,所有三個CDR)之重鏈;含有SEQ ID NO:12的一或更多CDR(例如,所有三個CDR)之輕鏈及含有SEQ ID NO:25的一或更多CDR(例如,所有三個CDR)之重鏈;含有SEQ ID NO:12的一或更多CDR(例如,所有三個CDR)之輕鏈及含有SEQ ID NO:137的一或更多CDR(例如,所有三個CDR)之重鏈;或含有SEQ ID NO:13的一或更多CDR(例如,所有三個CDR)之輕鏈及含有SEQ ID NO:26的一或更多CDR(例如,所有三個CDR)之重鏈序列。In a specific embodiment, the host cell comprises a nucleic acid (one or more nucleic acids) encoding a humanized light chain or a humanized heavy chain, wherein the humanized light chain and the humanized heavy chain together form a pair of human CD52 A specific binding humanized immunoglobulin and the humanized immunoglobulin thereof comprising a light chain comprising one or more CDRs of SEQ ID NO: 3 ( eg, all three CDRs) and one or more comprising SEQ ID NO: CDRs of more (e.g., all three CDR) of a heavy chain; comprising SEQ ID NO: CDRs of one or more (e.g., all three CDR) and the light chain of SEQ ID NO 4 comprising: 17 one or more CDRs of (e.g., all three CDR) of a heavy chain; comprising SEQ ID NO: CDRs of one or more (e.g., all three CDR) of 5 and a light chain comprising SEQ ID NO: 18 one or more of the CDRs of ( For example, a heavy chain of all three CDRs; a light chain comprising one or more CDRs of SEQ ID NO: 6 ( eg, all three CDRs) and one or more CDRs comprising SEQ ID NO: 19 ( eg, all a heavy chain of three CDRs; a light chain comprising one or more CDRs of SEQ ID NO: 7 ( eg, all three CDRs) and one or more CDRs comprising SEQ ID NO: 20 ( eg, all three Heavy chain of CDR); light chain comprising one or more CDRs of SEQ ID NO: 8 ( eg, all three CDRs) and one or more CDRs comprising SEQ ID NO: 21 ( eg, all three CDRs) Heavy chain; light chain comprising one or more CDRs of SEQ ID NO: 9 ( eg, all three CDRs) and one or more CDRs comprising SEQ ID NO: 22 ( eg, all three CDRs) chain; comprising SEQ ID NO: one or more CDR 10 (e.g., all three CDR) and the light chain comprises SEQ ID NO: CDRs of one or more (e.g., all three CDR) of the heavy chain 23 a light chain comprising one or more CDRs of SEQ ID NO: 11 (eg, all three CDRs) and a heavy chain comprising one or more CDRs of SEQ ID NO: 24 (eg, all three CDRs); a light chain of one or more CDRs (eg, all three CDRs) of SEQ ID NO: 12 and a heavy chain comprising one or more CDRs of SEQ ID NO: 25 ( eg , all three CDRs); comprising SEQ ID NO: one or more CDR 12 (e.g., all three CDR) and the light chain comprises SEQ ID NO: CDRs of one or more (e.g., all three CDR) of a heavy chain 137; or comprising SEQ ID NO : CDRs of one or more (e.g., all three CDR) of 13 and a light chain comprising SEQ ID NO: 26 CDRs of one or more (e.g., all three CDR) of the heavy chain sequence.

在一些具體實施例,該宿主細胞包含編碼人類化重鏈及人類化輕鏈的一或更多核酸分子,其中人類化輕鏈及人類化重鏈在一起會形成具對人類CD52的特定結合的人類化免疫球蛋白,其中該人類化免疫球蛋白結合至與老鼠單株抗體相同的位於人類CD52之抗原決定區,該老鼠單株抗體包含SEQ ID NO: 3的輕鏈變異區及SEQ ID NO: 16的重鏈變異區;SEQ ID NO:4的輕鏈變異區及SEQ ID NO: 17的重鏈變異區;SEQ ID NO: 5的輕鏈變異區及SEQ ID NO: 18的重鏈變異區;SEQ ID NO: 6的輕鏈變異區及SEQ ID NO: 19的重鏈變異區;SEQ ID NO: 7的輕鏈變異區及SEQ ID NO: 20的重鏈變異區;SEQ ID NO: 8的輕鏈變異區及SEQ ID NO: 21的重鏈變異區;SEQ ID NO: 9的輕鏈變異區及SEQ ID NO: 22的重鏈變異區;SEQ ID NO: 10的輕鏈變異區及SEQ ID NO: 23的重鏈變異區;SEQ ID NO: 11的輕鏈變異區及SEQ ID NO: 24的重鏈變異區;SEQ ID NO: 12的輕鏈變異區及SEQ ID NO: 25的重鏈變異區;或是SEQ ID NO: 13的輕鏈變異區及SEQ ID NO: 26的重鏈變異區。在其他具體實施例,該宿主細胞包含編碼人類化重鏈及人類化輕鏈的一或更多核酸分子,其中人類化輕鏈及人類化重鏈在一起會形成具對人類CD52的特定結合的人類化免疫球蛋白,其中該人類化免疫球蛋白結合至與此種老鼠單株抗體所結合抗原決定區重疊的人類CD52上的抗原決定區。In some embodiments, the host cell comprises one or more nucleic acid molecules encoding a humanized heavy chain and a humanized light chain, wherein the humanized light chain and the humanized heavy chain together form a specific binding to human CD52. A humanized immunoglobulin, wherein the humanized immunoglobulin binds to an epitope of human CD52 identical to a mouse monoclonal antibody comprising the light chain variant region of SEQ ID NO: 3 and SEQ ID NO : a heavy chain variant region of 16; a light chain variant region of SEQ ID NO: 4 and a heavy chain variant region of SEQ ID NO: 17; a light chain variant region of SEQ ID NO: 5 and a heavy chain variant of SEQ ID NO: Region; the light chain variant region of SEQ ID NO: 6 and the heavy chain variant region of SEQ ID NO: 19; the light chain variant region of SEQ ID NO: 7 and the heavy chain variant region of SEQ ID NO: 20; SEQ ID NO: a light chain variant region of 8 and a heavy chain variant region of SEQ ID NO: 21; a light chain variant region of SEQ ID NO: 9 and a heavy chain variant region of SEQ ID NO: 22; a light chain variant region of SEQ ID NO: And the heavy chain variation region of SEQ ID NO: 23; the light chain variation region of SEQ ID NO: 11 and the heavy chain variation region of SEQ ID NO: 24; The hetero region and the heavy chain variation region of SEQ ID NO: 25; or the light chain variation region of SEQ ID NO: 13 and the heavy chain variation region of SEQ ID NO: 26. In other specific embodiments, the host cell comprises one or more nucleic acid molecules encoding a humanized heavy chain and a humanized light chain, wherein the humanized light chain and the humanized heavy chain together form a specific binding to human CD52. A humanized immunoglobulin, wherein the humanized immunoglobulin binds to an epitope on human CD52 that overlaps with an epitope determined by the mouse monoclonal antibody.

在其他具體實施例,該宿主細胞包含編碼人類化重鏈及人類化輕鏈的一或更多核酸分子,其中人類化輕鏈及人類化重鏈在一起會形成具對人類CD52的特定結合的人類化免疫球蛋白,其中該人類化免疫球蛋白結合至包含至少成熟人類CD52的殘基1之抗原決定區;結合至包含至少成熟人類CD52的殘基1、3、4及5之抗原決定區;結合至包含至少成熟人類CD52的殘基1、2、3、4及5之抗原決定區;或是結合至包含至少成熟人類CD52的殘基7、8及9之抗原決定區。在一些具體實施例,該抗原決定區包含至少成熟人類CD52序列的殘基7、8及11。在一些具體實施例,該抗原決定區包含至少成熟人類CD52序列的殘基4及11。In other specific embodiments, the host cell comprises one or more nucleic acid molecules encoding a humanized heavy chain and a humanized light chain, wherein the humanized light chain and the humanized heavy chain together form a specific binding to human CD52. A humanized immunoglobulin, wherein the humanized immunoglobulin binds to an epitope comprising residue 1 of at least mature human CD52; binds to an epitope comprising residues 1, 3, 4 and 5 of at least mature human CD52 Binding to an epitope comprising residues 1, 2, 3, 4 and 5 of at least mature human CD52; or binding to an epitope comprising residues 7, 8 and 9 of at least mature human CD52. In some embodiments, the epitope comprises at least residues 7, 8 and 11 of the mature human CD52 sequence. In some embodiments, the epitope comprises at least residues 4 and 11 of the mature human CD52 sequence.

在一些具體實施例,該宿主細胞包含編碼人類化重鏈及人類化輕鏈的一或更多核酸分子,其中人類化輕鏈及人類化重鏈在一起會形成具對人類CD52的特定結合的人類化免疫球蛋白,其中該人類化免疫球蛋白包含一種輕鏈,其包含由SEQ ID NO: 115、SEQ ID NO: 118、及SEQ ID NO: 121所組成族群選出的一或更多CDR(例如,所有三個該CDR),及/或一種重鏈,其包含由SEQ ID NO: 124、SEQ ID NO: 127、及SEQ ID NO: 130所組成族群選出的一或更多CDR(例如,所有三個該CDR);一種輕鏈,其包含由SEQ ID NO: 116、SEQ ID NO: 119、及SEQ ID NO: 122所組成族群選出的一或更多CDR(例如,所有三個該CDR),及/或一種重鏈,其包含由SEQ ID NO: 125、SEQ ID NO: 128、及SEQ ID NO: 131所組成族群選出的一或更多CDR(例如,所有三個該CDR);或一種輕鏈,其包含由SEQ ID NO: 117、SEQ ID NO: 120、及SEQ ID NO: 123所組成族群選出的一或更多CDR(例如,所有三個該CDR),及/或一種重鏈,其包含由SEQ ID NO: 126、SEQ ID NO: 129、及SEQ ID NO: 132所組成族群選出的一或更多CDR(例如,所有三個該CDR)。In some embodiments, the host cell comprises one or more nucleic acid molecules encoding a humanized heavy chain and a humanized light chain, wherein the humanized light chain and the humanized heavy chain together form a specific binding to human CD52. A humanized immunoglobulin, wherein the humanized immunoglobulin comprises a light chain comprising one or more CDRs selected from the group consisting of SEQ ID NO: 115, SEQ ID NO: 118, and SEQ ID NO: 121 ( For example, all three of the CDRs, and/or a heavy chain comprising one or more CDRs selected from the group consisting of SEQ ID NO: 124, SEQ ID NO: 127, and SEQ ID NO: 130 ( eg, All three of the CDRs; a light chain comprising one or more CDRs selected from the group consisting of SEQ ID NO: 116, SEQ ID NO: 119, and SEQ ID NO: 122 ( eg, all three of the CDRs) And/or a heavy chain comprising one or more CDRs selected from the group consisting of SEQ ID NO: 125, SEQ ID NO: 128, and SEQ ID NO: 131 ( eg, all three of the CDRs); Or a light chain comprising one or more selected from the group consisting of SEQ ID NO: 117, SEQ ID NO: 120, and SEQ ID NO: 123 CDR (e.g., all three of the CDR), and / or one heavy chain comprising a SEQ ID NO: 126, SEQ ID NO: 129, and SEQ ID NO: 132 Suo one or more CDR selected from the group consisting of ( For example, all three of the CDRs).

在一些具體實施例,該宿主細胞包含編碼人類化重鏈及人類化輕鏈的一或更多核酸,其中人類化輕鏈及人類化重鏈在一起會形成具對人類CD52的特定結合的人類化免疫球蛋白,其中該人類化免疫球蛋白包含含有SEQ ID NO: 115、SEQ ID NO: 118及SEQ ID NO: 121的CDR之輕鏈及包含SEQ ID NO: 124、SEQ ID NO: 127及SEQ ID NO: 130的CDR之重鏈;包含SEQ ID NO: 116、SEQ ID NO: 119、及SEQ ID NO: 122的CDR之輕鏈及包含SEQ ID NO: 125、SEQ ID NO: 128及SEQ ID NO: 131的CDR之重鏈;或包含SEQ ID NO: 117、SEQ ID NO: 120及SEQ ID NO: 123的CDR之輕鏈及包含SEQ ID NO: 126、SEQ ID NO: 129及SEQ ID NO: 132的CDR之重鏈。In some embodiments, the host cell comprises one or more nucleic acids encoding a humanized heavy chain and a humanized light chain, wherein the humanized light chain and the humanized heavy chain together form a human having a specific binding to human CD52 An immunoglobulin comprising a light chain comprising the CDRs of SEQ ID NO: 115, SEQ ID NO: 118 and SEQ ID NO: 121 and comprising SEQ ID NO: 124, SEQ ID NO: 127 and a heavy chain of the CDRs of SEQ ID NO: 130; a light chain comprising the CDRs of SEQ ID NO: 116, SEQ ID NO: 119, and SEQ ID NO: 122 and comprising SEQ ID NO: 125, SEQ ID NO: 128, and SEQ ID NO: the heavy chain of the CDR of 131; or the light chain comprising the CDRs of SEQ ID NO: 117, SEQ ID NO: 120 and SEQ ID NO: 123 and comprising SEQ ID NO: 126, SEQ ID NO: 129 and SEQ ID NO: The heavy chain of the CDR of 132.

在其他具體實施例,該宿主細胞包含編碼人類化重鏈及人類化輕鏈的一或更多核酸分子,其中人類化輕鏈及人類化重鏈在一起會形成具對人類CD52的特定結合的人類化免疫球蛋白,其中該人類化免疫球蛋白對於醣化人類CD52較對於非-醣化或去-醣化人類CD52具有更大結合親和力,例如,顯現對醣化人類CD52特定的結合。人類化免疫球蛋白可結合至包含其N-鍵結碳水化合物基團的成熟人類CD52上的抗原決定區。此抗原決定區亦可包含至少成熟人類CD52序列的殘基1,至少成熟人類CD52序列的殘基3,至少成熟人類CD52序列的殘基1、3、4及5,或是至少成熟人類CD52序列的殘基1、2、3、4及5。In other specific embodiments, the host cell comprises one or more nucleic acid molecules encoding a humanized heavy chain and a humanized light chain, wherein the humanized light chain and the humanized heavy chain together form a specific binding to human CD52. Humanized immunoglobulins, wherein the humanized immunoglobulin has greater binding affinity for glycosylated human CD52 than for non-glycated or de-glycosylated human CD52, for example, exhibits specific binding to glycosylated human CD52. The humanized immunoglobulin can bind to an epitope on mature human CD52 comprising its N -bonded carbohydrate group. The epitope may also comprise at least residue 1 of the mature human CD52 sequence, at least residue 3 of the mature human CD52 sequence, at least residues 1, 3, 4 and 5 of the mature human CD52 sequence, or at least the mature human CD52 sequence. Residues 1, 2, 3, 4 and 5.

在一些具體實施例,該宿主細胞包含編碼人類化輕鏈的一種核酸分子,其包含SEQ ID NO:3、SEQ ID NO:4、SEQ ID NO:5、SEQ ID NO:6、SEQ ID NO:7、SEQ ID NO:8、SEQ ID NO:9、SEQ ID NO:10、SEQ ID NO:11、SEQ ID NO:12或SEQ ID NO:13的一或更多CDR(例如,所有三個CDR)。該人類化輕鏈不為Campath的人類化輕鏈。In some embodiments, the host cell comprises a nucleic acid molecule encoding a humanized light chain comprising SEQ ID NO:3, SEQ ID NO:4, SEQ ID NO:5, SEQ ID NO:6, SEQ ID NO: 7. One or more CDRs of SEQ ID NO: 8, SEQ ID NO: 9, SEQ ID NO: 10, SEQ ID NO: 11, SEQ ID NO: 12 or SEQ ID NO: 13 ( eg, all three CDRs) ). The humanized light chain is not for Campath Humanized light chain.

在其他具體實施例,該宿主細胞包含編碼人類化重鏈的一種核酸分子,其包含SEQ ID NO:16、SEQ ID NO:17、SEQ ID NO:18、SEQ ID NO:19、SEQ ID NO:20、SEQ ID NO:21、SEQ ID NO:22、SEQ ID NO:23、SEQ ID NO:24、SEQ ID NO:25、SEQ ID NO:26、或SEQ ID NO: 137的一或更多CDR(例如,所有三個CDR)。該人類化重鏈不為Campath的人類化重鏈。In other specific embodiments, the host cell comprises a nucleic acid molecule encoding a humanized heavy chain comprising SEQ ID NO: 16, SEQ ID NO: 17, SEQ ID NO: 18, SEQ ID NO: 19, SEQ ID NO: 20. One or more CDRs of SEQ ID NO: 21, SEQ ID NO: 22, SEQ ID NO: 23, SEQ ID NO: 24, SEQ ID NO: 25, SEQ ID NO: 26, or SEQ ID NO: 137 ( for example , all three CDRs). The humanized heavy chain is not for Campath Humanized heavy chain.

在一些具體實施例,該宿主細胞包含編碼人類化輕鏈的一種核酸,其中該人類化輕鏈包含由SEQ ID NO:27、SEQ ID NO:28、SEQ ID NO:29、SEQ ID NO:30、SEQ ID NO:31、SEQ ID NO:32、SEQ ID NO:33、SEQ ID NO:34、SEQ ID NO:35、SEQ ID NO:36、SEQ ID NO:37、SEQ ID NO:38、SEQ ID NO:39、SEQ ID NO:40、SEQ ID NO:41、SEQ ID NO:42、SEQ ID NO:43、SEQ ID NO:44、SEQ ID NO:45、SEQ ID NO:46、SEQ ID NO:47、及SEQ ID NO:48或是其組合所組成族群選出的一或更多CDR,其中該人類化輕鏈不為Campath的人類化輕鏈。In some embodiments, the host cell comprises a nucleic acid encoding a humanized light chain, wherein the humanized light chain comprises SEQ ID NO:27, SEQ ID NO:28, SEQ ID NO:29, SEQ ID NO:30 SEQ ID NO: 31, SEQ ID NO: 32, SEQ ID NO: 33, SEQ ID NO: 34, SEQ ID NO: 35, SEQ ID NO: 36, SEQ ID NO: 37, SEQ ID NO: 38, SEQ ID NO: 39, SEQ ID NO: 40, SEQ ID NO: 41, SEQ ID NO: 42, SEQ ID NO: 43, SEQ ID NO: 44, SEQ ID NO: 45, SEQ ID NO: 46, SEQ ID NO And one or more CDRs selected from the group consisting of: SEQ ID NO: 48 or a combination thereof, wherein the humanized light chain is not Campath Humanized light chain.

在其他具體實施例,該宿主細胞包含編碼人類化重鏈的一種核酸,其中該人類化重鏈包含由SEQ ID NO:49、SEQ ID NO:50、SEQ ID NO:51、SEQ ID NO:52、SEQ ID NO:53、SEQ ID NO:54、SEQ ID NO:55、SEQ ID NO:56、SEQ ID NO:57、SEQ ID NO:58、SEQ ID NO:59、SEQ ID NO:60、SEQ ID NO:61、SEQ ID NO:62、SEQ ID NO:63、SEQ ID NO:64、SEQ ID NO:65、SEQ ID NO:66、SEQ ID NO:67、SEQ ID NO:68、SEQ ID NO:69、SEQ ID NO:70、SEQ ID NO:71、SEQ ID NO:72、SEQ ID NO:73、SEQ ID NO:74、及SEQ ID NO: 294或是其組合所組成族群選出的一或更多CDR,其中該人類化重鏈不為Campath的人類化重鏈。In other specific embodiments, the host cell comprises a nucleic acid encoding a humanized heavy chain, wherein the humanized heavy chain comprises SEQ ID NO: 49, SEQ ID NO: 50, SEQ ID NO: 51, SEQ ID NO: 52 SEQ ID NO: 53, SEQ ID NO: 54, SEQ ID NO: 55, SEQ ID NO: 56, SEQ ID NO: 57, SEQ ID NO: 58, SEQ ID NO: 59, SEQ ID NO: 60, SEQ ID NO: 61, SEQ ID NO: 62, SEQ ID NO: 63, SEQ ID NO: 64, SEQ ID NO: 65, SEQ ID NO: 66, SEQ ID NO: 67, SEQ ID NO: 68, SEQ ID NO :69, one selected from the group consisting of SEQ ID NO: 70, SEQ ID NO: 71, SEQ ID NO: 72, SEQ ID NO: 73, SEQ ID NO: 74, and SEQ ID NO: 294, or a combination thereof More CDRs, where the humanized heavy chain is not Campath Humanized heavy chain.

本發明亦關於一種具對人類CD52的特定結合的人類化免疫球蛋白之製備方法,其包含在適合人類化免疫球蛋白表現的條件下培養本發明宿主細胞(例如,包含編碼本發明人類化免疫球蛋白(例如,本發明人類化輕鏈及人類化重鏈)的一或更多重組核酸之宿主細胞),藉以表現人類化免疫球蛋白鏈及製造人類化免疫球蛋白。在一些具體實施例,該方法進一步包含純化或分離人類化免疫球蛋白。在一些具體實施例,該方法進一步包含合併該經純化或分離人類化免疫球蛋白與生理上可接受媒劑或載體以製造醫藥組合物。The invention also relates to a method for the preparation of a humanized immunoglobulin having a specific binding to human CD52, comprising culturing a host cell of the invention under conditions suitable for the expression of a human immunoglobulin (eg, comprising encoding a humanized immunity of the invention) A host cell of one or more recombinant nucleic acids of a globulin (eg, a humanized light chain of the invention and a humanized heavy chain) whereby a humanized immunoglobulin chain is produced and a humanized immunoglobulin is produced. In some embodiments, the method further comprises purifying or isolating the humanized immunoglobulin. In some embodiments, the method further comprises combining the purified or isolated humanized immunoglobulin with a physiologically acceptable vehicle or carrier to produce a pharmaceutical composition.

本發明亦關於一種具對人類CD52的特定結合的人類化輕鏈之製備方法,其包含在適合人類化輕鏈表現的條件下培養本發明宿主細胞(例如,包含編碼本發明人類化輕鏈的一或更多重組核酸之宿主細胞),藉以表現人類化輕鏈及製造人類化輕鏈。在一些具體實施例,該方法進一步包含純化或分離人類化輕鏈。The invention also relates to a method of making a humanized light chain having a specific binding to human CD52 comprising culturing a host cell of the invention under conditions suitable for humanized light chain expression (eg, comprising a humanized light chain encoding the invention) One or more host cells for recombinant nucleic acid) to express humanized light chains and to make humanized light chains. In some embodiments, the method further comprises purifying or isolating the humanized light chain.

本發明亦關於一種具對人類CD52的特定結合的人類化重鏈之製備方法,其包含在適合人類化重鏈表現的條件下培養本發明宿主細胞(例如,包含編碼本發明人類化重鏈的一或更多重組核酸之宿主細胞),藉以表現人類化重鏈及製造人類化重鏈。在一些具體實施例,該方法進一步包含純化或分離人類化重鏈。The invention also relates to a method of making a humanized heavy chain having a specific binding to human CD52 comprising culturing a host cell of the invention under conditions suitable for humanized heavy chain expression (eg, comprising a humanized heavy chain encoding the invention) One or more host cells for recombinant nucleic acid) to express humanized heavy chains and to make humanized heavy chains. In some embodiments, the method further comprises purifying or isolating the humanized heavy chain.

本發明進一步關於一種醫藥組合物,其包含本發明人類化免疫球蛋白(例如,包含本發明人類化輕鏈及/或本發明人類化重鏈)及生理上可接受媒劑或載體。在一些具體實施例,該醫藥組合物包含一種單位劑量組合物。The invention further relates to a pharmaceutical composition comprising a humanized immunoglobulin of the invention (e.g., comprising a humanized light chain of the invention and/or a humanized heavy chain of the invention) and a physiologically acceptable vehicle or carrier. In some embodiments, the pharmaceutical composition comprises a unit dose composition.

本發明亦關於一種會分泌具對人類CD52的結合專一性的單株抗體之融合瘤細胞的製造方法,其包含將人類CD52的轉基因老鼠淋巴細胞至投與人類CD52轉基因老鼠相同或類似的族系(例如,CD1)的非-轉基因老鼠,藉以製造免疫、非-轉基因老鼠。該免疫,非-轉基因老鼠的脾細胞與永生細胞融合,藉以製造融合瘤細胞,該融合瘤細胞係培養在會分泌具對人類CD52的結合專一性的單株抗體之條件。在一些具體實施例,使用FACS分析以偵測會分泌具對人類CD52的結合專一性的單株抗體之融合瘤細胞。在其他具體實施例,轉基因老鼠族系及非-轉基因老鼠族系為相同的。在某些具體實施例,CD52為野生型人類CD52。在一些具體實施例,CD52轉基因老鼠及非-轉基因老鼠為CD1老鼠。在一些具體實施例,用於免疫的淋巴細胞係由人類CD52轉基因老鼠的脾臟得到。在一些具體實施例,永生細胞係由SP2/0 Ag14細胞及NS1骨髓瘤細胞所組成族群選出。本發明亦關於一種由本發明方法所製造的融合瘤細胞。選擇性地,收集由融合瘤細胞所分泌的單株抗體及進一步純化(例如,大體上純化,分離的)。在其他具體實施例,該方法進一步包含決定由融合瘤細胞所分泌的單株抗體之核苷酸序列。The present invention also relates to a method for producing a fusion tumor cell which secretes a monoclonal antibody having specificity for binding to human CD52, which comprises transgenic mouse lymphocytes of human CD52 to the same or similar families of human CD52 transgenic mice. Non-transgenic mice (eg, CD1) are used to make immune, non-transgenic mice. The immunized, non-transgenic mouse spleen cells were fused with immortal cells to produce fusion tumor cells cultured under conditions which secrete monoclonal antibodies having specificity for binding to human CD52. In some embodiments, FACS analysis is used to detect fusion tumor cells that secrete monoclonal antibodies with binding specificity for human CD52. In other embodiments, the transgenic mouse family and the non-transgenic mouse family are identical. In certain embodiments, CD52 is wild-type human CD52. In some embodiments, the CD52 transgenic mouse and the non-transgenic mouse are CD1 mice. In some embodiments, the lymphocyte line used for immunization is obtained from the spleen of a human CD52 transgenic mouse. In some embodiments, the immortalized cell line is selected from the group consisting of SP2/0 Ag14 cells and NS1 myeloma cells. The invention also relates to a fusion tumor cell made by the method of the invention. Alternatively, monoclonal antibodies secreted by the fusion tumor cells are collected and further purified (eg, substantially purified, isolated). In other embodiments, the method further comprises determining a nucleotide sequence of a monoclonal antibody secreted by the fusion tumor cell.

本發明亦關於一種於需要治療病人中自體免疫疾病(例如,多發性硬化症(MS)、類風濕關節炎(RA)(參看例如,Nature Reviews Drug Discovery 6: 75-92(2007))、血管炎(參看例如,Rheumatology 39:229-237(2000))、貝西氏病(BD)(參看例如,Rheumatology 42:1539-1544(2003))、狼瘡及乳糜瀉(Vivas,S.,等,N. Engl. J. Med.,354(23):2514-2515(2006))、血管炎、乾癬、肌炎、硬化症、再生障礙性貧血、及結腸炎)治療方法,其包含投藥有效量的本發明人類化免疫球蛋白至病人。The present invention also relates to an autoimmune disease (e.g., multiple sclerosis (MS), rheumatoid arthritis (RA) in a patient in need of treatment (see, for example, Nature Reviews Drug Discovery 6: 75-92 (2007)), Vasculitis (see, for example, Rheumatology 39: 229-237 (2000)), Beth's disease (BD) (see, for example, Rheumatology 42: 1539-1544 (2003)), lupus and celiac disease (Vivas, S., etc.) , N. Engl. J. Med. , 354(23): 2514-2515 (2006)), vasculitis, dryness, myositis, sclerosis, aplastic anemia, and colitis, including effective administration The amount of the human immunoglobulin of the invention is administered to a patient.

在另一方面,有效量的本發明人類化免疫球蛋白可與一或更多免疫抑制劑一起投藥以使需要此種治療的病人準備進行固體器官移植(AgarwalTransplant Immunol.,20:6-11(2008))或是CD34+幹細胞移植(Burt等,The Lancet,published online January 30,2009)。In another aspect, an effective amount of a humanized immunoglobulin of the invention can be administered with one or more immunosuppressive agents to prepare a patient for such treatment for solid organ transplantation (Agarwal et al , Transplant Immunol., 20: 6). -11 (2008)) or CD34+ stem cell transplantation (Burt et al, The Lancet, published online January 30, 2009).

本發明亦關於一種於需要治療病人的癌症治療方法,其包含投藥有效量的本發明人類化免疫球蛋白至病人。The invention also relates to a method of treating cancer in a patient in need thereof, comprising administering an effective amount of a humanized immunoglobulin of the invention to a patient.

本發明亦關於一種於需要治療病人的多發性硬化症治療方法,其包含投藥有效量的本發明人類化免疫球蛋白至病人。The invention also relates to a method of treating multiple sclerosis in a patient in need thereof, comprising administering an effective amount of a humanized immunoglobulin of the invention to a patient.

本發明亦關於一種於需要治療病人的慢性淋巴性白血病治療方法,其包含投藥有效量的本發明人類化免疫球蛋白至病人。The invention also relates to a method of treating chronic lymphocytic leukemia in a patient in need thereof, comprising administering an effective amount of a humanized immunoglobulin of the invention to a patient.

本發明人類化免疫球蛋白的投藥可包含(例如,於醫藥組合物)人類化免疫球蛋白本身的投藥,編碼人類化免疫球蛋白的一或更多重組載體之投藥,或是包含編碼人類化免疫球蛋白及表現人類化免疫球蛋白的一或更多核酸(例如,一或更多重組載體)的宿主細胞的投藥。The administration of the humanized immunoglobulin of the present invention may comprise (for example, in a pharmaceutical composition) administration of a humanized immunoglobulin itself, administration of one or more recombinant vectors encoding a humanized immunoglobulin, or inclusion of a coding humanization. Administration of an immunoglobulin and a host cell that exhibits one or more nucleic acids of a humanized immunoglobulin (eg, one or more recombinant vectors).

本發明亦關於一種由自體免疫疾病、癌症、非-何杰金氏淋巴瘤、多發性硬化症、狼瘡及慢性淋巴性白血病所組成族群選出的疾病之診斷方法,其包含使用本發明人類化免疫球蛋白活體外分析病人樣品。The present invention also relates to a method for diagnosing a disease selected from the group consisting of autoimmune diseases, cancer, non-Hodgkin's lymphoma, multiple sclerosis, lupus, and chronic lymphocytic leukemia, including humanization using the present invention Immunoglobulins are used to analyze patient samples in vitro.

本發明亦關於一種本發明人類化免疫球蛋白(例如,包含本發明人類化輕鏈及/或本發明人類化重鏈)、本發明重組載體、或是本發明宿主細胞,以用於藥物,例如用於治療及/或診斷疾病,例如用於治療此處所敘述疾病或失調例如自體免疫疾病(例如,多發性硬化症、類風濕關節炎、及狼瘡)、癌症、淋巴細胞超-增生情況(例如,包含白血病例如B-細胞慢性淋巴性白血病及淋巴瘤例如非-何杰金氏淋巴瘤的T或B細胞惡性腫瘤)。參考例如,Lundin,J.等,Blood,101:4267-4272(2003);Rodig,SJ.等,Clinical Cancer Research,12(23):7174-7179(2006)。本發明亦關於人類化免疫球蛋白、本發明人類化輕鏈或人類化重鏈、本發明重組載體、或是本發明宿主細胞的使用,以用於製造治療此處所敘述疾病或失調(例如,自體免疫疾病、癌症、非-何杰金氏淋巴瘤、多發性硬化症、慢性淋巴性白血病)的藥物。The invention also relates to a humanized immunoglobulin of the invention (for example comprising a humanized light chain of the invention and/or a humanized heavy chain of the invention), a recombinant vector of the invention, or a host cell of the invention for use in medicine, For example, for the treatment and/or diagnosis of diseases, for example for the treatment of diseases or disorders described herein such as autoimmune diseases (eg, multiple sclerosis, rheumatoid arthritis, and lupus), cancer, lymphocyte hyper-proliferation (For example, T or B cell malignancies comprising leukemia such as B-cell chronic lymphocytic leukemia and lymphoma such as non-Hodgkin's lymphoma). See, for example, Lundin, J. et al, Blood , 101: 4267-4272 (2003); Rodig, SJ. et al, Clinical Cancer Research, 12(23): 7174-7179 (2006). The invention also relates to the use of a humanized immunoglobulin, a humanized light chain or humanized heavy chain of the invention, a recombinant vector of the invention, or a host cell of the invention, for use in the manufacture of a disease or disorder described herein (eg, Drugs for autoimmune diseases, cancer, non-Hodgkin's lymphoma, multiple sclerosis, chronic lymphocytic leukemia.

老鼠單株免疫球蛋白Mouse monoclonal immunoglobulin

本發明亦關於具人類CD52結合專一性的老鼠單株抗體(老鼠單株免疫球蛋白)。在一個具體實施例,本發明係關於具人類CD52結合專一性的老鼠單株抗體,其包含含有SEQ ID NO: 3的輕鏈及含有SEQ ID NO: 16的重鏈;含有SEQ ID NO: 4的輕鏈及含有SEQ ID NO: 17的重鏈;含有SEQ ID NO: 5的輕鏈及含有SEQ ID NO: 18的重鏈;含有SEQ ID NO: 6的輕鏈及含有SEQ ID NO: 19的重鏈;含有SEQ ID NO: 7的輕鏈及含有SEQ ID NO: 20的重鏈;含有SEQ ID NO: 8的輕鏈及含有SEQ ID NO: 21的重鏈;含有SEQ ID NO: 9的輕鏈及含有SEQ ID NO: 22的重鏈;含有SEQI DN O: 10的輕鏈及含有SEQ ID NO: 23的重鏈;含有SEQ ID NO: 11的輕鏈及含有SEQ ID NO: 24的重鏈;含有SEQ ID NO: 12的輕鏈及含有SEQ ID NO: 25的重鏈或含有SEQ ID NO: 13的輕鏈及含有SEQ ID NO: 26的重鏈。The present invention also relates to a mouse monoclonal antibody (mouse monoclonal immunoglobulin) having human CD52 binding specificity. In a specific embodiment, the invention relates to a mouse monoclonal antibody having human CD52 binding specificity comprising a light chain comprising SEQ ID NO: 3 and a heavy chain comprising SEQ ID NO: 16; comprising SEQ ID NO: 4 a light chain and a heavy chain comprising SEQ ID NO: 17; a light chain comprising SEQ ID NO: 5 and a heavy chain comprising SEQ ID NO: 18; a light chain comprising SEQ ID NO: 6 and comprising SEQ ID NO: 19 Heavy chain; a light chain comprising SEQ ID NO: 7 and a heavy chain comprising SEQ ID NO: 20; a light chain comprising SEQ ID NO: 8 and a heavy chain comprising SEQ ID NO: 21; comprising SEQ ID NO: 9 a light chain and a heavy chain comprising SEQ ID NO: 22; a light chain comprising SESEQ DN O: 10 and a heavy chain comprising SEQ ID NO: 23; a light chain comprising SEQ ID NO: 11 and comprising SEQ ID NO: 24 Heavy chain; a light chain comprising SEQ ID NO: 12 and a heavy chain comprising SEQ ID NO: 25 or a light chain comprising SEQ ID NO: 13 and a heavy chain comprising SEQ ID NO: 26.

在一個具體實施例,具人類CD52結合專一性的老鼠單株抗體包含由SEQ ID NO:3、SEQ ID NO:4、SEQ ID NO:5、SEQ ID NO:6、SEQ ID NO:7、SEQ ID NO:8、SEQ ID NO:9、SEQ ID NO:10、SEQ ID NO:11、SEQ ID NO:12及SEQ ID NO:13所組成族群選出的輕鏈變異區,或是由SEQ ID NO:16、SEQ ID NO:17、SEQ ID NO:18、SEQ ID NO:19、SEQ ID NO:20、SEQ ID NO:21、SEQ ID NO:22、SEQ ID NO:23、SEQ ID NO:24、SEQ ID NO:25及SEQ ID NO:26所組成族群選出的重鏈變異區,或是此種輕鏈變異區及此種重鏈變異區皆包含。In a specific embodiment, the mouse monoclonal antibody having human CD52 binding specificity comprises SEQ ID NO: 3, SEQ ID NO: 4, SEQ ID NO: 5, SEQ ID NO: 6, SEQ ID NO: 7, SEQ ID NO: 8, a light chain variant region selected from the group consisting of SEQ ID NO: 9, SEQ ID NO: 10, SEQ ID NO: 11, SEQ ID NO: 12 and SEQ ID NO: 13, or by SEQ ID NO : 16, SEQ ID NO: 17, SEQ ID NO: 18, SEQ ID NO: 19, SEQ ID NO: 20, SEQ ID NO: 21, SEQ ID NO: 22, SEQ ID NO: 23, SEQ ID NO: 24. The heavy chain variation region selected from the group consisting of SEQ ID NO: 25 and SEQ ID NO: 26, or such a light chain variation region and such a heavy chain variation region are included.

本發明亦關於一種老鼠免疫球蛋白輕鏈,其包含SEQ ID NO:3、SEQ ID NO:4、SEQ ID NO:5、SEQ ID NO:6、SEQ ID NO:7、SEQ ID NO:8、SEQ ID NO:9、SEQ ID NO:10、SEQ ID NO:11、SEQ ID NO:12或SEQ ID NO:13的變異區。The invention also relates to a mouse immunoglobulin light chain comprising SEQ ID NO:3, SEQ ID NO:4, SEQ ID NO:5, SEQ ID NO:6, SEQ ID NO:7, SEQ ID NO:8, The variant region of SEQ ID NO: 9, SEQ ID NO: 10, SEQ ID NO: 11, SEQ ID NO: 12 or SEQ ID NO: 13.

本發明亦關於一種老鼠免疫球蛋白重鏈,其包含SEQ ID NO:16、SEQ ID NO:17、SEQ ID NO:18、SEQ ID NO:19、SEQ ID NO:20、SEQ ID NO:21、SEQ ID NO:22、SEQ ID NO:23、SEQ ID NO:24、SEQ ID NO:25或SEQ ID NO:26的變異區。The invention also relates to a mouse immunoglobulin heavy chain comprising SEQ ID NO: 16, SEQ ID NO: 17, SEQ ID NO: 18, SEQ ID NO: 19, SEQ ID NO: 20, SEQ ID NO: The variant region of SEQ ID NO:22, SEQ ID NO:23, SEQ ID NO:24, SEQ ID NO:25 or SEQ ID NO:26.

較佳為,本發明老鼠單株抗體包含本發明老鼠抗體輕鏈及本發明老鼠抗體重鏈。在一些具體實施例,本發明提供一種老鼠單株免疫球蛋白,其結合至與老鼠單株抗體相同的位於人類CD52之抗原決定區,其包含SEQ ID NO: 3的輕鏈變異區及SEQ ID NO: 16的重鏈變異區;SEQ ID NO: 4的輕鏈變異區及SEQ ID NO: 17的重鏈變異區;SEQ ID NO: 5的輕鏈變異區及SEQ ID NO: 18的重鏈變異區;SEQ ID NO: 6的輕鏈變異區及SEQ ID NO: 19的重鏈變異區;SEQ ID NO: 7的輕鏈變異區及SEQ ID NO: 20的重鏈變異區;SEQ ID NO: 8的輕鏈變異區及SEQ ID NO: 21的重鏈變異區;SEQ ID NO: 9的輕鏈變異區及SEQ ID NO: 22的重鏈變異區;SEQ ID NO: 10的輕鏈變異區及SEQ ID NO: 23的重鏈變異區;SEQ ID NO: 11的輕鏈變異區及SEQ ID NO: 24的重鏈變異區;SEQ ID NO: 12的輕鏈變異區及SEQ ID NO: 25的重鏈變異區;或是SEQ ID NO: 13的輕鏈變異區及SEQ ID NO: 26的重鏈變異區。在其他具體實施例,本發明提供一種老鼠單株免疫球蛋白,其結合至人類CD52上的抗原決定區,其與老鼠單株抗體所結合的抗原決定區重疊。Preferably, the mouse monoclonal antibody of the present invention comprises the mouse antibody light chain of the present invention and the mouse antibody heavy chain of the present invention. In some embodiments, the invention provides a mouse monoclonal immunoglobulin that binds to an epitope of human CD52 identical to a mouse monoclonal antibody, comprising the light chain variant region of SEQ ID NO: 3 and the SEQ ID a heavy chain variant region of NO: 16; a light chain variant region of SEQ ID NO: 4; and a heavy chain variant region of SEQ ID NO: 17; a light chain variant region of SEQ ID NO: 5 and a heavy chain of SEQ ID NO: Variant region; light chain variant region of SEQ ID NO: 6 and heavy chain variant region of SEQ ID NO: 19; light chain variant region of SEQ ID NO: 7 and heavy chain variant region of SEQ ID NO: 20; SEQ ID NO a light chain variant region of 8 and a heavy chain variant region of SEQ ID NO: 21; a light chain variant region of SEQ ID NO: 9 and a heavy chain variant region of SEQ ID NO: 22; light chain variation of SEQ ID NO: a region and a heavy chain variant region of SEQ ID NO: 23; a light chain variant region of SEQ ID NO: 11 and a heavy chain variant region of SEQ ID NO: 24; a light chain variant region of SEQ ID NO: 12 and SEQ ID NO: a heavy chain variant region of 25; or a light chain variant region of SEQ ID NO: 13 and a heavy chain variant region of SEQ ID NO: 26. In other embodiments, the invention provides a mouse monoclonal immunoglobulin that binds to an epitope on human CD52 that overlaps with an epitope determined by a mouse monoclonal antibody.

在其他具體實施例,本發明提供一種老鼠單株免疫球蛋白,其結合至人類CD52上的抗原決定區,其包含至少成熟人類CD52序列的殘基1。該老鼠單株免疫球蛋白可結合至包含至少成熟人類CD52序列的殘基1、3、4及5之抗原決定區,可結合至包含至少成熟人類CD52序列的殘基1、2、3、4及5之抗原決定區,或是可結合至包含至少成熟人類CD52序列的殘基7、8及9之抗原決定區。在一些具體實施例,該抗原決定區包含至少成熟人類CD52序列的殘基7、8及11。在一些具體實施例,該抗原決定區包含至少成熟人類CD52序列的殘基4及11。In other specific embodiments, the invention provides a mouse monoclonal immunoglobulin that binds to an epitope of human CD52 comprising at least residue 1 of a mature human CD52 sequence. The mouse monoclonal immunoglobulin can bind to an epitope comprising residues 1, 3, 4 and 5 of at least the mature human CD52 sequence, and can bind to residues 1, 2, 3, 4 comprising at least the mature human CD52 sequence. And an epitope of 5, or an epitope determined to bind to residues 7, 8 and 9 of at least the mature human CD52 sequence. In some embodiments, the epitope comprises at least residues 7, 8 and 11 of the mature human CD52 sequence. In some embodiments, the epitope comprises at least residues 4 and 11 of the mature human CD52 sequence.

本發明亦關於一種經分離核酸分子,其編碼本發明老鼠單株免疫球蛋白、老鼠免疫球蛋白輕鏈或老鼠免疫球蛋白重鏈。在一些具體實施例,本發明為一種經分離核酸分子,其編碼老鼠免疫球蛋白重鏈及老鼠免疫球蛋白輕鏈,它們在一起會形成具對人類CD52的特定結合的老鼠單株免疫球蛋白,其中該老鼠免疫球蛋白輕鏈包含由SEQ ID NO:3、SEQ ID NO:4、SEQ ID NO:5、SEQ ID NO:6、SEQ ID NO:7、SEQ ID NO:8、SEQ ID NO:9、SEQ ID NO:10、SEQ ID NO:11、SEQ ID NO:12及SEQ ID NO:13所組成族群選出的變異區,或是該老鼠免疫球蛋白重鏈包含由SEQ ID NO:16、SEQ ID NO:17、SEQ ID NO:18、SEQ ID NO:19、SEQ ID NO:20、SEQ ID NO:21、SEQ ID NO:22、SEQ ID NO:23、SEQ ID NO:24、SEQ ID NO:25及SEQ ID NO:26所組成族群選出的變異區,或是此種輕鏈及此種重鏈皆包含。The invention also relates to an isolated nucleic acid molecule encoding a mouse monoclonal immunoglobulin, a mouse immunoglobulin light chain or a mouse immunoglobulin heavy chain of the invention. In some embodiments, the invention is an isolated nucleic acid molecule encoding a mouse immunoglobulin heavy chain and a mouse immunoglobulin light chain which together form a mouse monoclonal immunoglobulin having a specific binding to human CD52 Wherein the mouse immunoglobulin light chain comprises SEQ ID NO: 3, SEQ ID NO: 4, SEQ ID NO: 5, SEQ ID NO: 6, SEQ ID NO: 7, SEQ ID NO: 8, SEQ ID NO a variant region selected from the group consisting of SEQ ID NO: 10, SEQ ID NO: 11, SEQ ID NO: 12 and SEQ ID NO: 13, or the mouse immunoglobulin heavy chain comprising SEQ ID NO: SEQ ID NO: 17, SEQ ID NO: 18, SEQ ID NO: 19, SEQ ID NO: 20, SEQ ID NO: 21, SEQ ID NO: 22, SEQ ID NO: 23, SEQ ID NO: 24, SEQ ID NO: 25 and the variant region selected by the group consisting of SEQ ID NO: 26, or such a light chain and such a heavy chain are included.

在一些具體實施例,該經分離核酸編碼老鼠免疫球蛋白輕鏈,其包含由SEQ ID NO:3、SEQ ID NO:4、SEQ ID NO:5、SEQ ID NO:6、SEQ ID NO:7、SEQ ID NO:8、SEQ ID NO:9、SEQ ID NO:10、SEQ ID NO:11、SEQ ID NO:12及SEQ ID NO:13所組成族群選出的變異區。In some embodiments, the isolated nucleic acid encodes a mouse immunoglobulin light chain comprising SEQ ID NO:3, SEQ ID NO:4, SEQ ID NO:5, SEQ ID NO:6, SEQ ID NO:7 The variant regions selected from the group consisting of SEQ ID NO: 8, SEQ ID NO: 9, SEQ ID NO: 10, SEQ ID NO: 11, SEQ ID NO: 12, and SEQ ID NO: 13.

在其他具體實施例,該經分離核酸編碼老鼠免疫球蛋白重鏈,其包含由SEQ ID NO:16、SEQ ID NO:17、SEQ ID NO:18、SEQ ID NO:19、SEQ ID NO:20、SEQ ID NO:21、SEQ ID NO:22、SEQ ID NO:23、SEQ ID NO:24、SEQ ID NO:25及SEQ ID NO:26所組成族群選出的變異區。In other specific embodiments, the isolated nucleic acid encodes a mouse immunoglobulin heavy chain comprising SEQ ID NO: 16, SEQ ID NO: 17, SEQ ID NO: 18, SEQ ID NO: 19, SEQ ID NO: The variant regions selected from the group consisting of SEQ ID NO: 21, SEQ ID NO: 22, SEQ ID NO: 23, SEQ ID NO: 24, SEQ ID NO: 25, and SEQ ID NO: 26.

本發明亦相關於一種重組載體(例如,表現載體,其包含哺乳動物細胞表現載體),其包含編碼本發明老鼠單株免疫球蛋白(例如,老鼠免疫球蛋白輕鏈及老鼠免疫球蛋白重鏈)、老鼠免疫球蛋白輕鏈、或老鼠免疫球蛋白重鏈的核酸。在一些具體實施例,本發明為包含編碼老鼠單株免疫球蛋白的核酸的一種重組載體,或一對包含編碼老鼠單株免疫球蛋白的核酸的重組載體,其包含由SEQ ID NO:3、SEQ ID NO:4、SEQ ID NO:5、SEQ ID NO:6、SEQ ID NO:7、SEQ ID NO:8、SEQ ID NO:9、SEQ ID NO:10、SEQ ID NO:11、SEQ ID NO:12及SEQ ID NO:13所組成族群選出的輕鏈變異區,或由SEQ ID NO:16、SEQ ID NO:17、SEQ ID NO:18、SEQ ID NO:19、SEQ ID NO:20、SEQ ID NO:21、SEQ ID NO:22、SEQ ID NO:23、SEQ ID NO:24、SEQ ID NO:25及SEQ ID NO:26所組成族群選出的重鏈變異區,或是此種輕鏈變異區及此種重鏈變異區皆包含。The invention also relates to a recombinant vector ( e.g. , an expression vector comprising a mammalian cell expression vector) comprising a mouse monoclonal immunoglobulin encoding the invention (e.g., a mouse immunoglobulin light chain and a mouse immunoglobulin heavy chain) ), a mouse immunoglobulin light chain, or a nucleic acid of a mouse immunoglobulin heavy chain. In some embodiments, the invention is a recombinant vector comprising a nucleic acid encoding a mouse monoclonal immunoglobulin, or a pair of recombinant vectors comprising a nucleic acid encoding a mouse monoclonal immunoglobulin comprising SEQ ID NO:3, SEQ ID NO:4, SEQ ID NO:5, SEQ ID NO:6, SEQ ID NO:7, SEQ ID NO:8, SEQ ID NO:9, SEQ ID NO:10, SEQ ID NO:11, SEQ ID a light chain variant region selected from the group consisting of NO: 12 and SEQ ID NO: 13, or SEQ ID NO: 16, SEQ ID NO: 17, SEQ ID NO: 18, SEQ ID NO: 19, SEQ ID NO: 20. a heavy chain variant region selected from the group consisting of SEQ ID NO: 21, SEQ ID NO: 22, SEQ ID NO: 23, SEQ ID NO: 24, SEQ ID NO: 25, and SEQ ID NO: 26, or Both the light chain variant region and the heavy chain variant region are included.

在其他具體實施例,該重組載體包含編碼老鼠免疫球蛋白輕鏈的核酸,其中該老鼠免疫球蛋白輕鏈包含SEQ ID NO:3、SEQ ID NO:4、SEQ ID NO:5、SEQ ID NO:6、SEQ ID NO:7、SEQ ID NO:8、SEQ ID NO:9、SEQ ID NO:10、SEQ ID NO:11、SEQ ID NO:12或SEQ ID NO:13。In other specific embodiments, the recombinant vector comprises a nucleic acid encoding a mouse immunoglobulin light chain, wherein the mouse immunoglobulin light chain comprises SEQ ID NO:3, SEQ ID NO:4, SEQ ID NO:5, SEQ ID NO : SEQ ID NO: 7, SEQ ID NO: 8, SEQ ID NO: 9, SEQ ID NO: 10, SEQ ID NO: 11, SEQ ID NO: 12 or SEQ ID NO: 13.

在其他具體實施例,該重組載體包含編碼老鼠免疫球蛋白重鏈的核酸,其中該老鼠免疫球蛋白重鏈包含SEQ ID NO:16、SEQ ID NO:17、SEQ ID NO:18、SEQ ID NO:19、SEQ ID NO:20、SEQ ID NO:21、SEQ ID NO:22、SEQ ID NO:23、SEQ ID NO:24、SEQ ID NO:25或SEQ ID NO:26。In other specific embodiments, the recombinant vector comprises a nucleic acid encoding a mouse immunoglobulin heavy chain, wherein the mouse immunoglobulin heavy chain comprises SEQ ID NO: 16, SEQ ID NO: 17, SEQ ID NO: 18, SEQ ID NO : 19, SEQ ID NO: 20, SEQ ID NO: 21, SEQ ID NO: 22, SEQ ID NO: 23, SEQ ID NO: 24, SEQ ID NO: 25 or SEQ ID NO: 26.

在其他具體實施例,該重組載體包含編碼老鼠免疫球蛋白輕鏈及老鼠免疫球蛋白重鏈的核酸,其中該老鼠免疫球蛋白輕鏈及老鼠免疫球蛋白重鏈在一起會形成具對人類CD52的特定結合的老鼠單株免疫球蛋白。在一個具體實施例,該老鼠免疫球蛋白輕鏈包含由SEQ ID NO:3、SEQ ID NO:4、SEQ ID NO:5、SEQ ID NO:6、SEQ ID NO:7、SEQ ID NO: 8、SEQ ID NO: 9、SEQ ID NO: 10、SEQ ID NO: 11、SEQ ID NO: 12及SEQ ID NO: 13所組成族群選出的變異區,及該老鼠單株免疫球蛋白重鏈包含由SEQ ID NO: 16、SEQ ID NO: 17、SEQ ID NO: 18、SEQ ID NO: 19、SEQ ID NO: 20、SEQ ID NO: 21、SEQ ID NO: 22、SEQ ID NO: 23、SEQ ID NO: 24、SEQ ID NO: 25及SEQ ID NO: 26所組成族群選出的變異區。In other specific embodiments, the recombinant vector comprises a nucleic acid encoding a mouse immunoglobulin light chain and a mouse immunoglobulin heavy chain, wherein the mouse immunoglobulin light chain and the mouse immunoglobulin heavy chain together form a pair of human CD52 Specific binding of mouse monoclonal immunoglobulin. In a specific embodiment, the mouse immunoglobulin light chain comprises SEQ ID NO:3, SEQ ID NO:4, SEQ ID NO:5, SEQ ID NO:6, SEQ ID NO:7, SEQ ID NO:8 a variant region selected from the group consisting of SEQ ID NO: 9, SEQ ID NO: 10, SEQ ID NO: 11, SEQ ID NO: 12, and SEQ ID NO: 13, and the mouse immunoglobulin heavy chain comprising SEQ ID NO: 16, SEQ ID NO: 17, SEQ ID NO: 18, SEQ ID NO: 19, SEQ ID NO: 20, SEQ ID NO: 21, SEQ ID NO: 22, SEQ ID NO: 23, SEQ ID NO: 24, a variant region selected from the group consisting of SEQ ID NO: 25 and SEQ ID NO: 26.

在特定具體實施例,本發明重組載體為一種表現載體,例如哺乳動物細胞表現載體。在某些具體實施例,載體係為一種質粒或是病毒載體(例如,腺病毒或AAV載體)。In a specific embodiment, the recombinant vector of the invention is a performance vector, such as a mammalian cell expression vector. In certain embodiments, the vector is a plasmid or a viral vector ( eg , an adenovirus or an AAV vector).

本發明亦關於一種宿主細胞,其包含一種編碼本發明老鼠單株免疫球蛋白(老鼠免疫球蛋白輕鏈及老鼠免疫球蛋白重鏈)、老鼠免疫球蛋白輕鏈或老鼠單株免疫球蛋白重鏈的一或更多核酸。例如,在一些具體實施例,該宿主細胞包含一種本發明重組載體(例如,表現載體,哺乳動物細胞表現載體)。The invention also relates to a host cell comprising a mouse monoclonal immunoglobulin (mouse immunoglobulin light chain and mouse immunoglobulin heavy chain), mouse immunoglobulin light chain or mouse immunoglobulin weight One or more nucleic acids of the chain. For example, in some embodiments, the host cell comprises a recombinant vector of the invention ( e.g. , an expression vector, a mammalian cell expression vector).

在一些具體實施例,該宿主細胞包含一種編碼老鼠免疫球蛋白輕鏈及老鼠免疫球蛋白重鏈的核酸,其中該老鼠免疫球蛋白輕鏈及該老鼠免疫球蛋白重鏈在一起會形成具對人類CD52的特定結合的老鼠單株免疫球蛋白及其中該老鼠免疫球蛋白輕鏈包含由SEQ ID NO: 3、SEQ ID NO: 4、SEQ ID NO: 5、SEQ ID NO: 6、SEQ ID NO: 7、SEQ ID NO: 8、SEQ ID NO: 9、SEQ ID NO: 10、SEQ ID NO: 11、SEQ ID NO: 12及SEQ ID NO: 13所組成族群選出的變異區,及/或該老鼠免疫球蛋白重鏈包含由SEQ ID NO:16、SEQ ID NO:17、SEQ ID NO:18、SEQ ID NO:19、SEQ ID NO:20、SEQ ID NO:21、SEQ ID NO:22、SEQ ID NO:23、SEQ ID NO:24、SEQ ID NO:25及SEQ ID NO:26所組成族群選出的變異區,或二者皆具。In some embodiments, the host cell comprises a nucleic acid encoding a mouse immunoglobulin light chain and a mouse immunoglobulin heavy chain, wherein the mouse immunoglobulin light chain and the mouse immunoglobulin heavy chain together form a pair Specific binding mouse monoclonal immunoglobulin of human CD52 and the mouse immunoglobulin light chain thereof comprising SEQ ID NO: 3, SEQ ID NO: 4, SEQ ID NO: 5, SEQ ID NO: 6, SEQ ID NO a variant region selected from the group consisting of SEQ ID NO: 8, SEQ ID NO: 9, SEQ ID NO: 10, SEQ ID NO: 11, SEQ ID NO: 12, and SEQ ID NO: 13, and/or The mouse immunoglobulin heavy chain comprises SEQ ID NO: 16, SEQ ID NO: 17, SEQ ID NO: 18, SEQ ID NO: 19, SEQ ID NO: 20, SEQ ID NO: 21, SEQ ID NO: The variant regions selected by the population consisting of SEQ ID NO: 23, SEQ ID NO: 24, SEQ ID NO: 25 and SEQ ID NO: 26, or both.

在一些具體實施例,該宿主細胞包含一種編碼老鼠免疫球蛋白輕鏈的核酸,其中該老鼠免疫球蛋白輕鏈包含由SEQ ID NO:3、SEQ ID NO:4、SEQ ID NO:5、SEQ ID NO:6、SEQ ID NO:7、SEQ ID NO:8、SEQ ID NO:9、SEQ ID NO:10、SEQ ID NO:11、SEQ ID NO:12及SEQ ID NO:13所組成族群選出的輕鏈變異區。In some embodiments, the host cell comprises a nucleic acid encoding a mouse immunoglobulin light chain, wherein the mouse immunoglobulin light chain comprises SEQ ID NO:3, SEQ ID NO:4, SEQ ID NO:5, SEQ ID NO:6, SEQ ID NO:7, SEQ ID NO:8, SEQ ID NO:9, SEQ ID NO:10, SEQ ID NO:11, SEQ ID NO:12, and SEQ ID NO:13 Light chain variation region.

在一些具體實施例,該宿主細胞包含一種編碼老鼠免疫球蛋白重鏈的核酸,其中該老鼠免疫球蛋白重鏈包含由SEQ ID NO:16、SEQ ID NO:17、SEQ ID NO:18、SEQ ID NO:19、SEQ ID NO:20、SEQ ID NO:21、SEQ ID NO:22、SEQ ID NO:23、SEQ ID NO:24、SEQ ID NO:25及SEQ ID NO:26所組成族群選出的重鏈變異區。In some embodiments, the host cell comprises a nucleic acid encoding a mouse immunoglobulin heavy chain, wherein the mouse immunoglobulin heavy chain comprises SEQ ID NO: 16, SEQ ID NO: 17, SEQ ID NO: 18, SEQ Selected groups consisting of ID NO: 19, SEQ ID NO: 20, SEQ ID NO: 21, SEQ ID NO: 22, SEQ ID NO: 23, SEQ ID NO: 24, SEQ ID NO: 25, and SEQ ID NO: Heavy chain variation region.

本發明亦關於一種老鼠單株免疫球蛋白之製備方法,其包含在適合老鼠單株免疫球蛋白表現的條件下培養本發明宿主細胞(例如,包含編碼本發明老鼠單株免疫球蛋白(例如,老鼠免疫球蛋白輕鏈及老鼠免疫球蛋白重鏈)的一或更多重組核酸(例如,重組載體)之宿主細胞),藉以表現老鼠單株免疫球蛋白鏈及製造老鼠單株免疫球蛋白。在一些具體實施例,該方法進一步包含純化或分離老鼠單株免疫球蛋白。The present invention also relates to a method for producing a mouse monoclonal immunoglobulin comprising culturing a host cell of the present invention under conditions suitable for the expression of a mouse monoclonal immunoglobulin ( for example, comprising a mouse monoclonal immunoglobulin encoding the present invention (for example, A host cell of one or more recombinant nucleic acids (eg, a recombinant vector) of a mouse immunoglobulin light chain and a mouse immunoglobulin heavy chain), thereby expressing a mouse monoclonal immunoglobulin chain and producing a mouse monoclonal immunoglobulin. In some embodiments, the method further comprises purifying or isolating the mouse monoclonal immunoglobulin.

本發明亦關於一種老鼠單株免疫球蛋白輕鏈之製備方法,其包含在適合該老鼠免疫球蛋白輕鏈表現的條件下培養本發明宿主細胞(包含編碼本發明老鼠免疫球蛋白輕鏈的核酸),藉以表現輕鏈。在一些具體實施例,該方法進一步包含純化或分離該輕鏈。The invention also relates to a method for preparing a mouse monoclonal immunoglobulin light chain comprising culturing a host cell of the invention (including a nucleic acid encoding the mouse immunoglobulin light chain of the invention) under conditions suitable for the expression of the immunoglobulin light chain of the mouse ), in order to express the light chain. In some embodiments, the method further comprises purifying or isolating the light chain.

本發明亦關於一種老鼠單株免疫球蛋白重鏈之製備方法,其包含在適合該老鼠免疫球蛋白重鏈表現的條件下培養本發明宿主細胞(包含編碼本發明老鼠免疫球蛋白重鏈的核酸),藉以表現老鼠免疫球蛋白重鏈。在一些具體實施例,該方法進一步包含純化或分離該老鼠免疫球蛋白重鏈。The invention also relates to a method for preparing a mouse monoclonal immunoglobulin heavy chain comprising culturing a host cell of the invention (containing a nucleic acid encoding a mouse immunoglobulin heavy chain of the invention under conditions suitable for expression of the immunoglobulin heavy chain of the mouse) ), in order to express the mouse immunoglobulin heavy chain. In some embodiments, the method further comprises purifying or isolating the mouse immunoglobulin heavy chain.

本發明亦關於一種疾病診斷方法(例如,自體免疫疾病、癌症、非-何杰金氏淋巴瘤、多發性硬化症及慢性淋巴性白血病),其包含使用本發明老鼠單株免疫球蛋白活體外分析病人樣品(例如,Lundin,J.Blood,101:4267-4272(2003);Rodig,SJ等,Clin. Cancer res.,12(23);7174-717179(2006))。The present invention also relates to a disease diagnosis method (for example, autoimmune disease, cancer, non-Hodgkin's lymphoma, multiple sclerosis, and chronic lymphocytic leukemia), which comprises using the mouse monoclonal immunoglobulin living body of the present invention. Patient samples are analyzed externally (e.g., Lundin, J. et al , Blood, 101: 4267-4272 (2003); Rodig, SJ et al, Clin. Cancer res ., 12(23); 7174-717179 (2006)).

嵌合免疫球蛋白Chimeric immunoglobulin

本發明亦關於一種具對人類CD52的特定結合的嵌合免疫球蛋白,此種嵌合免疫球蛋白可包含本發明任何老鼠單株免疫球蛋白的變異區。在一個具體實施例,本發明嵌合免疫球蛋白包含SEQ ID NO: 3的輕鏈變異區及SEQ ID NO: 16的重鏈變異區;SEQ ID NO: 4的輕鏈變異區及SEQ ID NO: 17的重鏈變異區;SEQ ID NO: 5的輕鏈變異區及SEQ ID NO: 18的重鏈變異區;SEQ ID NO: 6的輕鏈變異區及SEQ ID NO: 19的重鏈變異區;SEQ ID NO: 7的輕鏈變異區及SEQ ID NO: 20的重鏈變異區;SEQ ID NO: 8的輕鏈變異區及SEQ ID NO: 21的重鏈變異區;SEQ ID NO: 9的輕鏈變異區及SEQ ID NO: 22的重鏈變異區;SEQ ID NO: 10的輕鏈變異區及SEQ ID NO: 23的重鏈變異區;SEQ ID NO: 11的輕鏈變異區及SEQ ID NO: 24的重鏈變異區;SEQ ID NO: 12的輕鏈變異區及SEQ ID NO: 25的重鏈變異區;或是SEQ ID NO: 13的輕鏈變異區及SEQ ID NO: 26的重鏈變異區。The invention also relates to a chimeric immunoglobulin having a specific binding to human CD52, which chimeric immunoglobulin may comprise a variant region of any mouse monoclonal immunoglobulin of the invention. In a specific embodiment, the chimeric immunoglobulin of the invention comprises the light chain variant region of SEQ ID NO: 3 and the heavy chain variant region of SEQ ID NO: 16; the light chain variant region of SEQ ID NO: 4 and SEQ ID NO : a heavy chain variant region of 17; a light chain variant region of SEQ ID NO: 5 and a heavy chain variant region of SEQ ID NO: 18; a light chain variant region of SEQ ID NO: 6 and a heavy chain variant of SEQ ID NO: Region; the light chain variant region of SEQ ID NO: 7 and the heavy chain variant region of SEQ ID NO: 20; the light chain variant region of SEQ ID NO: 8 and the heavy chain variant region of SEQ ID NO: 21; SEQ ID NO: a light chain variant region of 9 and a heavy chain variant region of SEQ ID NO: 22; a light chain variant region of SEQ ID NO: 10 and a heavy chain variant region of SEQ ID NO: 23; a light chain variant region of SEQ ID NO: And the heavy chain variant region of SEQ ID NO: 24; the light chain variant region of SEQ ID NO: 12 and the heavy chain variant region of SEQ ID NO: 25; or the light chain variant region of SEQ ID NO: 13 and SEQ ID NO : 26 heavy chain variation regions.

本發明亦關於一種具對人類CD52的特定結合的嵌合免疫球蛋白,其包含由下列所組成族群選出的輕鏈變異區序列:SEQ ID NO: 3的輕鏈變異區、SEQ ID NO: 4的輕鏈變異區、SEQ ID NO: 5的輕鏈變異區、SEQ ID NO: 6的輕鏈變異區、SEQ ID NO: 7的輕鏈變異區、SEQ ID NO: 8的輕鏈變異區、SEQ ID NO: 9的輕鏈變異區、SEQ ID NO: 10的輕鏈變異區、SEQ ID NO: 11的輕鏈變異區、SEQ ID NO: 12的輕鏈變異區及SEQ ID NO: 13的輕鏈變異區,及/或由下列所組成族群選出的重鏈變異區序列:SEQ ID NO: 16的重鏈變異區、SEQ ID NO: 17的重鏈變異區、SEQ ID NO: 18的重鏈變異區、SEQ ID NO: 19的重鏈變異區、SEQ ID NO: 20的重鏈變異區、SEQ ID NO: 21的重鏈變異區、SEQ ID NO: 22的重鏈變異區、SEQ ID NO: 23的重鏈變異區、SEQ ID NO: 24的重鏈變異區、SEQ ID NO: 25的重鏈變異區及SEQ ID NO: 26的重鏈變異區。The invention also relates to a chimeric immunoglobulin having a specific binding to human CD52 comprising a sequence of a light chain variant region selected from the group consisting of: a light chain variant region of SEQ ID NO: 3, SEQ ID NO: 4 a light chain variant region, a light chain variant region of SEQ ID NO: 5, a light chain variant region of SEQ ID NO: 6, a light chain variant region of SEQ ID NO: 7, a light chain variant region of SEQ ID NO: 8, The light chain variant region of SEQ ID NO: 9, the light chain variant region of SEQ ID NO: 10, the light chain variant region of SEQ ID NO: 11, the light chain variant region of SEQ ID NO: 12, and the SEQ ID NO: 13 a light chain variant region, and/or a heavy chain variant region sequence selected from the group consisting of: the heavy chain variant region of SEQ ID NO: 16, the heavy chain variant region of SEQ ID NO: 17, and the weight of SEQ ID NO: 18. The chain variant region, the heavy chain variant region of SEQ ID NO: 19, the heavy chain variant region of SEQ ID NO: 20, the heavy chain variant region of SEQ ID NO: 21, the heavy chain variant region of SEQ ID NO: 22, SEQ ID NO: a heavy chain variant region of 23, a heavy chain variant region of SEQ ID NO: 24, a heavy chain variant region of SEQ ID NO: 25, and a heavy chain variant region of SEQ ID NO: 26.

本發明亦關於一種嵌合輕鏈,其包含由SEQ ID NO:3、SEQ ID NO:4、SEQ ID NO:5、SEQ ID NO:6、SEQ ID NO:7、SEQ ID NO:8、SEQ ID NO:9、SEQ ID NO:10、SEQ ID NO:11、SEQ ID NO:12及SEQ ID NO:13所組成族群選出的變異區。The invention also relates to a chimeric light chain comprising SEQ ID NO: 3, SEQ ID NO: 4, SEQ ID NO: 5, SEQ ID NO: 6, SEQ ID NO: 7, SEQ ID NO: 8, SEQ ID NO: 9, a variant region selected from the group consisting of SEQ ID NO: 10, SEQ ID NO: 11, SEQ ID NO: 12, and SEQ ID NO: 13.

本發明亦關於一種嵌合重鏈,其包含由SEQ ID NO:16、SEQ ID NO:17、SEQ ID NO:18、SEQ ID NO:19、SEQ ID NO:20、SEQ ID NO:21、SEQ ID NO:22、SEQ ID NO:23、SEQ ID NO:24、SEQ ID NO:25及SEQ ID NO:26所組成族群選出的變異區。The invention also relates to a chimeric heavy chain comprising SEQ ID NO: 16, SEQ ID NO: 17, SEQ ID NO: 18, SEQ ID NO: 19, SEQ ID NO: 20, SEQ ID NO: 21, SEQ ID NO: 22, SEQ ID NO: 23, SEQ ID NO: 24, SEQ ID NO: 25, and SEQ ID NO: 26 selected variant regions.

較佳為,本發明嵌合免疫球蛋白包含本發明嵌合輕鏈及本發明嵌合重鏈。Preferably, the chimeric immunoglobulins of the invention comprise a chimeric light chain of the invention and a chimeric heavy chain of the invention.

在一些具體實施例,本發明提供一種結合至與老鼠單株抗體相同的位於人類CD52之抗原決定區的嵌合免疫球蛋白,其包含SEQ ID NO: 3的輕鏈變異區及SEQ ID NO: 16的重鏈變異區;SEQ ID NO: 4的輕鏈變異區及SEQ ID NO: 17的重鏈變異區;SEQ ID NO: 5的輕鏈變異區及SEQ ID NO: 18的重鏈變異區;SEQ ID NO: 6的輕鏈變異區及SEQ ID NO: 19的重鏈變異區;SEQ ID NO: 7的輕鏈變異區及SEQ ID NO: 20的重鏈變異區;SEQ ID NO: 8的輕鏈變異區及SEQ ID NO: 21的重鏈變異區;SEQ ID NO: 9的輕鏈變異區及SEQ ID NO: 22的重鏈變異區;SEQ ID NO:10的輕鏈變異區及SEQ ID NO: 23的重鏈變異區;SEQ ID NO: 11的輕鏈變異區及SEQ ID NO: 24的重鏈變異區;SEQ ID NO: 12的輕鏈變異區及SEQ ID NO: 25的重鏈變異區;或是SEQ ID NO: 13的輕鏈變異區及SEQ ID NO: 26的重鏈變異區。在其他具體實施例,該嵌合免疫球蛋白結合至於人類CD52上的抗原決定區,此抗原決定區與老鼠單株抗體所結合的抗原決定區重疊。In some embodiments, the invention provides a chimeric immunoglobulin that binds to an epitope of human CD52 that is identical to a mouse monoclonal antibody, comprising the light chain variant region of SEQ ID NO: 3 and SEQ ID NO: a heavy chain variant region of 16; a light chain variant region of SEQ ID NO: 4 and a heavy chain variant region of SEQ ID NO: 17; a light chain variant region of SEQ ID NO: 5 and a heavy chain variant region of SEQ ID NO: ; the light chain variant region of SEQ ID NO: 6 and the heavy chain variant region of SEQ ID NO: 19; the light chain variant region of SEQ ID NO: 7 and the heavy chain variant region of SEQ ID NO: 20; SEQ ID NO: 8 a light chain variant region and a heavy chain variant region of SEQ ID NO: 21; a light chain variant region of SEQ ID NO: 9 and a heavy chain variant region of SEQ ID NO: 22; a light chain variant region of SEQ ID NO: 10 and The heavy chain variant region of SEQ ID NO: 23; the light chain variant region of SEQ ID NO: 11 and the heavy chain variant region of SEQ ID NO: 24; the light chain variant region of SEQ ID NO: 12 and SEQ ID NO: The heavy chain variant region; or the light chain variant region of SEQ ID NO: 13 and the heavy chain variant region of SEQ ID NO: 26. In other embodiments, the chimeric immunoglobulin binds to an epitope of human CD52 that overlaps with an epitope determined by a mouse monoclonal antibody.

在其他具體實施例,本發明提供一種嵌合免疫球蛋白,其結合至人類CD52上的抗原決定區,其包含至少成熟人類CD52序列的殘基1。該嵌合免疫球蛋白可結合至包含至少成熟人類CD52序列的殘基1、3、4及5之抗原決定區,可結合至包含至少成熟人類CD52序列的殘基1、2、3、4及5之抗原決定區,或是可結合至包含至少成熟人類CD52序列的殘基7、8及9之抗原決定區於人類CD52上。在一些具體實施例,該抗原決定區包含至少成熟人類CD52序列的殘基7、8及11。在一些具體實施例,該抗原決定區包含至少成熟人類CD52序列的殘基4及11。In other specific embodiments, the invention provides a chimeric immunoglobulin that binds to an epitope of human CD52 comprising at least residue 1 of a mature human CD52 sequence. The chimeric immunoglobulin can bind to an epitope comprising residues 1, 3, 4 and 5 of at least the mature human CD52 sequence, and can bind to residues 1, 2, 3, 4 comprising at least the mature human CD52 sequence and An epitope of 5, or an epitope that binds to residues 7, 8 and 9 comprising at least the mature human CD52 sequence on human CD52. In some embodiments, the epitope comprises at least residues 7, 8 and 11 of the mature human CD52 sequence. In some embodiments, the epitope comprises at least residues 4 and 11 of the mature human CD52 sequence.

本發明亦關於一種經分離核酸分子,其編碼本發明嵌合免疫球蛋白、嵌合輕鏈或嵌合重鏈。在一些具體實施例,本發明為一種編碼嵌合重鏈及嵌合輕鏈的經分離核酸分子(一或更多核酸分子),嵌合重鏈及嵌合輕鏈在一起會形成具對人類CD52的特定結合的嵌合免疫球蛋白,其中該嵌合輕鏈包含由SEQ ID NO:3、SEQ ID NO:4、SEQ ID NO:5、SEQ ID NO:6、SEQ ID NO:7、SEQ ID NO:8、SEQ ID NO: 9、SEQ ID NO: 10、SEQ ID NO: 11、SEQ ID NO: 12及SEQ ID NO: 13所組成族群選出的變異區;及/或該嵌合重鏈包含由SEQ ID NO: 16、SEQ ID NO: 17、SEQ ID NO:18、SEQ ID NO: 19、SEQ ID NO: 20、SEQ ID NO:21、SEQ ID NO: 22、SEQ ID NO: 23、SEQ ID NO: 24、SEQ ID NO: 25及SEQ ID NO: 26所組成族群選出的變異區。The invention also relates to an isolated nucleic acid molecule encoding a chimeric immunoglobulin, chimeric light chain or chimeric heavy chain of the invention. In some embodiments, the invention is an isolated nucleic acid molecule (one or more nucleic acid molecules) encoding a chimeric heavy chain and a chimeric light chain, the chimeric heavy chain and the chimeric light chain together forming a pair of human A specific binding chimeric immunoglobulin of CD52, wherein the chimeric light chain comprises SEQ ID NO:3, SEQ ID NO:4, SEQ ID NO:5, SEQ ID NO:6, SEQ ID NO:7, SEQ ID NO: 8, a variant region selected from the group consisting of SEQ ID NO: 9, SEQ ID NO: 10, SEQ ID NO: 11, SEQ ID NO: 12, and SEQ ID NO: 13; and/or the chimeric heavy chain Including SEQ ID NO: 16, SEQ ID NO: 17, SEQ ID NO: 18, SEQ ID NO: 19, SEQ ID NO: 20, SEQ ID NO: 21, SEQ ID NO: 22, SEQ ID NO: 23. The variant regions selected from the group consisting of SEQ ID NO: 24, SEQ ID NO: 25 and SEQ ID NO: 26.

在一些具體實施例,本發明為一種編碼嵌合輕鏈的經分離核酸分子,嵌合輕鏈包含SEQ ID NO:3、SEQ ID NO:4、SEQ ID NO:5、SEQ ID NO:6、SEQ ID NO:7、SEQ ID NO:8、SEQ ID NO:9、SEQ ID NO:10、SEQ ID NO:11、SEQ ID NO:12或SEQ ID NO:13的變異區。In some embodiments, the invention is an isolated nucleic acid molecule encoding a chimeric light chain comprising SEQ ID NO:3, SEQ ID NO:4, SEQ ID NO:5, SEQ ID NO:6, The variant region of SEQ ID NO: 7, SEQ ID NO: 8, SEQ ID NO: 9, SEQ ID NO: 10, SEQ ID NO: 11, SEQ ID NO: 12 or SEQ ID NO: 13.

在一些具體實施例,本發明為一種編碼嵌合重鏈的經分離核酸分子,嵌合重鏈包含SEQ ID NO:16、SEQ ID NO:17、SEQ ID NO:18、SEQ ID NO:19、SEQ ID NO:20、SEQ ID NO:21、SEQ ID NO:22、SEQ ID NO:23、SEQ ID NO:24、SEQ ID NO:25或SEQ ID NO:26的變異區。In some embodiments, the invention is an isolated nucleic acid molecule encoding a chimeric heavy chain comprising SEQ ID NO: 16, SEQ ID NO: 17, SEQ ID NO: 18, SEQ ID NO: The variant region of SEQ ID NO:20, SEQ ID NO:21, SEQ ID NO:22, SEQ ID NO:23, SEQ ID NO:24, SEQ ID NO:25 or SEQ ID NO:26.

本發明亦相關於一種重組載體(例如,表現載體,哺乳動物細胞表現載體),其包含編碼本發明嵌合免疫球蛋白(嵌合輕鏈及嵌合重鏈)、嵌合輕鏈、或嵌合重鏈的核酸。在一些具體實施例,本發明為一種包含編碼嵌合免疫球蛋白的一種核酸的重組載體(或包含核酸的一對重組載體),其包含由SEQ ID NO:3、SEQ ID NO:4、SEQ ID NO:5、SEQ ID NO:6、SEQ ID NO:7、SEQ ID NO:8、SEQ ID NO:9、SEQ ID NO:10、SEQ ID NO:11、SEQ ID NO:12及SEQ ID NO:13所組成族群選出的輕鏈變異區;或由SEQ ID NO:16、SEQ ID NO:17、SEQ ID NO:18、SEQ ID NO:19、SEQ ID NO:20、SEQ ID NO:21、SEQ ID NO:22、SEQ ID NO:23、SEQ ID NO:24、SEQ ID NO:25及SEQ ID NO:26所組成族群選出的重鏈變異區;或此種輕鏈及重鏈皆具。The invention also relates to a recombinant vector ( e.g., expression vector, mammalian cell expression vector) comprising a chimeric immunoglobulin (chimeric light chain and chimeric heavy chain) encoding a chimeric light chain, chimeric light chain, or embedded A nucleic acid of a heavy chain. In some embodiments, the invention is a recombinant vector (or a pair of recombinant vectors comprising a nucleic acid) comprising a nucleic acid encoding a chimeric immunoglobulin comprising SEQ ID NO: 3, SEQ ID NO: 4, SEQ ID NO: 5, SEQ ID NO: 6, SEQ ID NO: 7, SEQ ID NO: 8, SEQ ID NO: 9, SEQ ID NO: 10, SEQ ID NO: 11, SEQ ID NO: 12, and SEQ ID NO : a light chain variant region selected from the group consisting of 13; or SEQ ID NO: 16, SEQ ID NO: 17, SEQ ID NO: 18, SEQ ID NO: 19, SEQ ID NO: 20, SEQ ID NO: 21, The heavy chain variant regions selected from the group consisting of SEQ ID NO: 22, SEQ ID NO: 23, SEQ ID NO: 24, SEQ ID NO: 25, and SEQ ID NO: 26; or such light and heavy chains.

在其他具體實施例,該重組載體包含編碼嵌合輕鏈的核酸,其中該嵌合輕鏈包含SEQ ID NO:3、SEQ ID NO:4、SEQ ID NO:5、SEQ ID NO:6、SEQ ID NO:7、SEQ ID NO:8、SEQ ID NO:9、SEQ ID NO:10、SEQ ID NO:11、SEQ ID NO:12或SEQ ID NO:13的變異區。In other specific embodiments, the recombinant vector comprises a nucleic acid encoding a chimeric light chain, wherein the chimeric light chain comprises SEQ ID NO:3, SEQ ID NO:4, SEQ ID NO:5, SEQ ID NO:6, SEQ ID NO: 7, variant region of SEQ ID NO: 8, SEQ ID NO: 9, SEQ ID NO: 10, SEQ ID NO: 11, SEQ ID NO: 12 or SEQ ID NO: 13.

在其他具體實施例,該重組載體包含編碼嵌合重鏈的核酸,其中該嵌合重鏈包含SEQ ID NO:16、SEQ ID NO:17、SEQ ID NO:18、SEQ ID NO:19、SEQ ID NO:20、SEQ ID NO:21、SEQ ID NO:22、SEQ ID NO:23、SEQ ID NO:24、SEQ ID NO:25或SEQ ID NO:26的變異區。In other specific embodiments, the recombinant vector comprises a nucleic acid encoding a chimeric heavy chain, wherein the chimeric heavy chain comprises SEQ ID NO: 16, SEQ ID NO: 17, SEQ ID NO: 18, SEQ ID NO: 19, SEQ ID NO: 20, SEQ ID NO: 21, SEQ ID NO: 22, SEQ ID NO: 23, SEQ ID NO: 24, SEQ ID NO: 25 or SEQ ID NO: 26.

在特定具體實施例,本發明重組載體為一種表現載體,例如哺乳動物細胞表現載體。在某些具體實施例,載體係為一種質粒或是病毒載體(例如,腺病毒或AAV載體)。In a specific embodiment, the recombinant vector of the invention is a performance vector, such as a mammalian cell expression vector. In certain embodiments, the vector is a plasmid or a viral vector ( eg , an adenovirus or an AAV vector).

本發明亦相關於一種包含編碼本發明嵌合免疫球蛋白(嵌合輕鏈及嵌合重鏈)、嵌合輕鏈或嵌合重鏈的一或更多核酸(例如,一或更多重組載體)的宿主細胞。例如,在一些具體實施例,宿主細胞包含一種本發明重組載體(例如,表現載體,哺乳動物細胞表現載體)。The invention also relates to a nucleic acid comprising one or more nucleic acids encoding a chimeric immunoglobulin (chimeric light chain and chimeric heavy chain), chimeric light chain or chimeric heavy chain of the invention ( eg , one or more recombinants) Host cell of the vector). For example, in some embodiments, the host cell comprises a recombinant vector of the invention ( e.g. , a performance vector, a mammalian cell expression vector).

在一些具體實施例,該宿主細胞包含編碼嵌合輕鏈及嵌合重鏈的一種重組核酸(或一對重組核酸),其中該嵌合輕鏈及該嵌合重鏈在一起會形成具對人類CD52的結合專一性的嵌合免疫球蛋白,其中該嵌合輕鏈包含由SEQ ID NO:3、SEQ ID NO:4、SEQ ID NO:5、SEQ ID NO:6、SEQ ID NO:7、SEQ ID NO:8、SEQ ID NO:9、SEQ ID NO:10、SEQ ID NO:11、SEQ ID NO:12及SEQ ID NO:13所組成族群選出的變異區;及/或該嵌合重鏈包含由SEQ ID NO:16、SEQ ID NO:17、SEQ ID NO:18、SEQ ID NO:19、SEQ ID NO:20、SEQ ID NO:21、SEQ ID NO:22、SEQ ID NO:23、SEQ ID NO:24、SEQ ID NO:25及SEQ ID NO:26所組成族群選出的變異區。In some embodiments, the host cell comprises a recombinant nucleic acid (or a pair of recombinant nucleic acids) encoding a chimeric light chain and a chimeric heavy chain, wherein the chimeric light chain and the chimeric heavy chain together form a pair A chimeric immunoglobulin that binds to a specificity of human CD52, wherein the chimeric light chain comprises SEQ ID NO: 3, SEQ ID NO: 4, SEQ ID NO: 5, SEQ ID NO: 6, SEQ ID NO: 7. a variant region selected from the group consisting of SEQ ID NO: 8, SEQ ID NO: 9, SEQ ID NO: 10, SEQ ID NO: 11, SEQ ID NO: 12, and SEQ ID NO: 13; The heavy chain comprises SEQ ID NO: 16, SEQ ID NO: 17, SEQ ID NO: 18, SEQ ID NO: 19, SEQ ID NO: 20, SEQ ID NO: 21, SEQ ID NO: 22, SEQ ID NO: 23. A variant region selected from the group consisting of SEQ ID NO: 24, SEQ ID NO: 25 and SEQ ID NO: 26.

在一些具體實施例,該宿主細胞包含編碼嵌合輕鏈的重組核酸,其中該嵌合輕鏈包含由SEQ ID NO:3、SEQ ID NO:4、SEQ ID NO:5、SEQ ID NO:6、SEQ ID NO:7、SEQ ID NO:8、SEQ ID NO:9、SEQ ID NO:10、SEQ ID NO:11、SEQ ID NO:12、及SEQ ID NO:13所組成族群選出的輕鏈變異區。In some embodiments, the host cell comprises a recombinant nucleic acid encoding a chimeric light chain, wherein the chimeric light chain comprises SEQ ID NO:3, SEQ ID NO:4, SEQ ID NO:5, SEQ ID NO:6 , light chain selected from the group consisting of SEQ ID NO: 7, SEQ ID NO: 8, SEQ ID NO: 9, SEQ ID NO: 10, SEQ ID NO: 11, SEQ ID NO: 12, and SEQ ID NO: Variation zone.

在一些具體實施例,該宿主細胞包含編碼嵌合重鏈的重組核酸,其中該嵌合重鏈包含由SEQ ID NO:16、SEQ ID NO:17、SEQ ID NO:18、SEQ ID NO:19、SEQ ID NO:20、SEQ ID NO:21、SEQ ID NO:22、SEQ ID NO:23、SEQ ID NO:24、SEQ ID NO:25及SEQ ID NO:26所組成族群選出的重鏈變異區。In some embodiments, the host cell comprises a recombinant nucleic acid encoding a chimeric heavy chain, wherein the chimeric heavy chain comprises SEQ ID NO:16, SEQ ID NO:17, SEQ ID NO:18, SEQ ID NO:19 Heavy chain variants selected from the group consisting of SEQ ID NO: 20, SEQ ID NO: 21, SEQ ID NO: 22, SEQ ID NO: 23, SEQ ID NO: 24, SEQ ID NO: 25, and SEQ ID NO: Area.

本發明亦關於一種嵌合免疫球蛋白之製備方法,其包含在適合嵌合免疫球蛋白表現的條件下培養本發明宿主細胞(例如,包含編碼本發明嵌合免疫球蛋白(例如,嵌合輕鏈及嵌合重鏈)的一或更多經分離核酸的宿主細胞),藉以表現嵌合免疫球蛋白鏈及製造嵌合免疫球蛋白。在一些具體實施例,該方法進一步包含純化或分離嵌合免疫球蛋白。The invention also relates to a method of making a chimeric immunoglobulin comprising culturing a host cell of the invention under conditions suitable for expression of a chimeric immunoglobulin (e.g., comprising a chimeric immunoglobulin encoding the invention (e.g., chimeric light) The chain and the chimeric heavy chain) are one or more host cells from which the nucleic acid is isolated, thereby expressing the chimeric immunoglobulin chain and making the chimeric immunoglobulin. In some embodiments, the method further comprises purifying or isolating the chimeric immunoglobulin.

本發明亦關於一種嵌合輕鏈之製備方法,其包含在適合該嵌合輕鏈表現的條件下培養本發明宿主細胞(例如,包含編碼本發明嵌合輕鏈的核酸之宿主細胞),藉以表現嵌合輕鏈及製造嵌合輕鏈。在一些具體實施例,該方法進一步包含純化或分離該嵌合輕鏈。The invention also relates to a method of making a chimeric light chain comprising culturing a host cell of the invention (e.g., a host cell comprising a nucleic acid encoding a chimeric light chain of the invention) under conditions suitable for expression of the chimeric light chain, thereby The chimeric light chain is expressed and the chimeric light chain is produced. In some embodiments, the method further comprises purifying or isolating the chimeric light chain.

本發明亦關於一種嵌合重鏈之製備方法,其包含在適合該嵌合重鏈表現的條件下培養本發明宿主細胞(例如,包含編碼本發明嵌合重鏈的核酸之宿主細胞),藉以表現嵌合重鏈及製造嵌合重鏈。在一些具體實施例,該方法進一步包含純化或分離該嵌合重鏈。The invention also relates to a method of making a chimeric heavy chain comprising culturing a host cell of the invention (e.g., a host cell comprising a nucleic acid encoding a chimeric heavy chain of the invention) under conditions suitable for the performance of the chimeric heavy chain, thereby The chimeric heavy chain is expressed and the chimeric heavy chain is produced. In some embodiments, the method further comprises purifying or isolating the chimeric heavy chain.

本發明亦關於一種由自體免疫疾病、癌症、非-何杰金氏淋巴瘤、多發性硬化症及慢性淋巴性白血病所組成族群選出的疾病之診斷方法,其包含使用本發明嵌合免疫球蛋白活體外分析病人樣品。The present invention also relates to a method for diagnosing a disease selected from the group consisting of autoimmune diseases, cancer, non-Hodgkin's lymphoma, multiple sclerosis, and chronic lymphocytic leukemia, comprising using the chimeric immunosphere of the present invention Protein samples were analyzed in vitro for patient samples.

本發明亦關於一種單株抗-人類CD52抗體或其抗原-結合部分,其中該抗體的輕鏈及重鏈所包含三個互補決定區段(CDR)的發現是:分別在SEQ ID NO: 3及16;分別在SEQ ID NO: 4及17;分別在SEQ ID NO: 5及18;分別在SEQ ID NO: 6及19;分別在SEQ ID NO: 7及20;分別在SEQ ID NO: 8及21;分別在SEQ ID NO: 9及22;分別在SEQ ID NO: 10及23;分別在SEQ ID NO: 11及24;分別在SEQ ID NO: 12及25;分別在SEQ ID NO: 12及137;或分別在SEQ ID NO: 13及26。在一些具體實施例,本發明亦關於一種結合至與上文單株抗體或抗原-結合部分相同的位於人類CD52抗體之抗原決定區。在一些具體實施例,本發明亦關於一種與上文單株抗體或抗原-結合部分競爭的抗體。在一些具體實施例,本發明亦關於一種與上文單株抗體或抗原-結合部分互相競爭的抗體。The invention also relates to a monoclonal anti-human CD52 antibody or antigen - binding portion thereof, wherein the light and heavy chains of the antibody comprise three complementarity determining regions (CDRs) found in SEQ ID NO: 3, respectively. And 16; SEQ ID NOS: 4 and 17; SEQ ID NOS: 5 and 18, respectively; SEQ ID NOS: 6 and 19, respectively; SEQ ID NOS: 7 and 20, respectively; SEQ ID NO: 8 And 21; SEQ ID NOS: 9 and 22, respectively; SEQ ID NOS: 10 and 23, respectively; SEQ ID NOS: 11 and 24, respectively; SEQ ID NOS: 12 and 25, respectively; SEQ ID NO: 12, respectively. And 137; or SEQ ID NOS: 13 and 26, respectively. In some embodiments, the invention also relates to an epitope-binding region of a human CD52 antibody that binds to the same monoclonal antibody or antigen-binding portion as above. In some embodiments, the invention also relates to an antibody that competes with a monoclonal antibody or antigen-binding portion as described above. In some embodiments, the invention also relates to an antibody that competes with a monoclonal antibody or antigen-binding portion of the above.

在一些具體實施例,任何上文抗體或抗原-結合部分結合至包含SEQ ID NO: 104的胺基酸序列,及該抗體或部分至SEQ ID NO: 104的結合係由在SEQ ID NO: 104的殘基4、7、8、或11的丙胺酸取代所還原。In some embodiments, any of the above antibodies or antigen-binding portions bind to an amino acid sequence comprising SEQ ID NO: 104, and the antibody or portion to SEQ ID NO: 104 is SEQ ID NO: 104 The residue of the residue 4, 7, 8, or 11 is reduced by alanine substitution.

在一些具體實施例,抗體係為一種人類化抗體、老鼠抗體、或嵌合抗體。在某些具體實施例,該抗體重鏈的骨架區利用VH3-72或VH3-23人類生殖株序列及該抗體輕鏈的骨架區利用VK2 A18b人類生殖株序列。In some embodiments, the anti-system is a humanized antibody, a mouse antibody, or a chimeric antibody. In certain embodiments, the framework region of the antibody heavy chain utilizes the VH3-72 or VH3-23 human reproductive strain sequence and the framework region of the antibody light chain utilizes the VK2 A18b human reproductive strain sequence.

在一些具體實施例,本發明係關於一種單株抗-人類CD52抗體或其抗原-結合部分,其中該抗體包含重鏈(H)-CDR1、H-CDR2、H-CDR3,輕鏈(L)-CDR1、L-CDR2、及L-CDR3,其胺基酸序列分別為SEQ ID NO: 51、59、69、29、36及43;分別為SEQ ID NO: 50、60、69、29、37及43;分別為SEQ ID NO: 50、61、68、29、38及43;分別為SEQ ID NO: 50、61、69、29、36及43;分別為SEQ ID NO: 50、62、69、29、39及43;分別為SEQ ID NO: 52、61、70、30、40及43;分別為SEQ ID NO: 53、63、71、31、36及44;分別為SEQ ID NO: 54、64、71、31、36及45;分別為SEQ ID NO: 55、63、72、31、36及46;分別為SEQ ID NO: 56、65、73、32、41及47;分別為SEQ ID NO: 56、65、294、32、41及47;或分別為SEQ ID NO: 56、66、74、33、41及48。In some embodiments, the invention relates to a monoclonal anti-human CD52 antibody or antigen-binding portion thereof, wherein the antibody comprises a heavy chain (H)-CDR1, H-CDR2, H-CDR3, and a light chain (L) - CDR1, L-CDR2, and L-CDR3, the amino acid sequences of which are SEQ ID NOs: 51, 59, 69, 29, 36, and 43, respectively; SEQ ID NOs: 50, 60, 69, 29, 37, respectively And 43; SEQ ID NOs: 50, 61, 68, 29, 38 and 43; SEQ ID NOs: 50, 61, 69, 29, 36 and 43; SEQ ID NO: 50, 62, 69, respectively , 29, 39 and 43; SEQ ID NO: 52, 61, 70, 30, 40 and 43; SEQ ID NO: 53, 63, 71, 31, 36 and 44, respectively; SEQ ID NO: 54 , 64, 71, 31, 36 and 45; SEQ ID NOs: 55, 63, 72, 31, 36 and 46; SEQ ID NOs: 56, 65, 73, 32, 41 and 47, respectively; ID NO: 56, 65, 294, 32, 41 and 47; or SEQ ID NOS: 56, 66, 74, 33, 41 and 48, respectively.

在一些具體實施例,本發明係關於一種單株抗-人類CD52抗體或其抗原-結合部分,其中該抗體輕鏈及重鏈分別包含SEQ ID NO: 3及16;分別包含SEQ ID NO: 4及17;分別包含SEQ ID NO: 5及18;分別包含SEQ ID NO: 6及19;分別包含SEQ ID NO: 7及20;分別包含SEQ ID NO: 8及21;分別包含SEQ ID NO: 9及22;分別包含SEQ ID NO: 10及23;分別包含SEQ ID NO: 11及24;分別包含SEQ ID NO: 12及25或分別包含SEQ ID NO: 13及26的胺基酸序列。In some embodiments, the invention relates to a monoclonal anti-human CD52 antibody or antigen-binding portion thereof, wherein the antibody light and heavy chains comprise SEQ ID NOs: 3 and 16, respectively; SEQ ID NO: 4, respectively And 17; comprising SEQ ID NOS: 5 and 18, respectively; SEQ ID NOS: 6 and 19, respectively; SEQ ID NOS: 7 and 20, respectively; SEQ ID NOS: 8 and 21, respectively; SEQ ID NO: 9 respectively And 22; comprising SEQ ID NOS: 10 and 23, respectively; SEQ ID NOS: 11 and 24, respectively; SEQ ID NOS: 12 and 25, respectively, or amino acid sequences comprising SEQ ID NOS: 13 and 26, respectively.

在一些具體實施例,本發明係關於一種單株抗體或其抗原-結合部分,其中該抗體的重鏈及輕鏈分別包含SEQ ID NO: 103及102;分別包含SEQ ID NO: 136及138;分別包含SEQ ID NO: 137及138;分別包含SEQ ID NO: 139及147;分別包含SEQ ID NOs: 149及155;分別包含SEQ ID NO: 149及156;分別包含SEQ ID NO: 158及165;分別包含SEQ ID NO: 158及166;分別包含SEQ ID NO: 159及165;分別包含SEQ ID NO: 159及166;分別包含SEQ ID NO: 161及166;或分別包含SEQ ID NO: 163及166的胺基酸序列。在一些具體實施例,本發明係關於一種結合至與上述單株抗體或其抗原-結合部分相同的位於人類CD52之抗體的抗原決定區。在一些具體實施例,本發明係關於一種與上述單株抗體或其抗原-結合部分競爭之抗體。在一些具體實施例,本發明係關於一種與上述單株抗體或其抗原-結合部分交互競爭之抗體。In some embodiments, the invention relates to a monoclonal antibody or an antigen-binding portion thereof, wherein the heavy and light chains of the antibody comprise SEQ ID NOS: 103 and 102, respectively; SEQ ID NOS: 136 and 138, respectively; SEQ ID NO: 137 and 138, respectively; SEQ ID NO: 139 and 147, respectively; SEQ ID NO: 149 and 155, respectively; SEQ ID NO: 149 and 156, respectively; SEQ ID NO: 158 and 165, respectively; SEQ ID NO: 158 and 166, respectively; SEQ ID NO: 159 and 165, respectively; SEQ ID NO: 159 and 166, respectively; SEQ ID NO: 161 and 166, respectively; or SEQ ID NO: 163 and 166, respectively Amino acid sequence. In some embodiments, the invention relates to an epitope determined to bind to an antibody to human CD52 that is identical to the monoclonal antibody or antigen-binding portion thereof described above. In some embodiments, the invention relates to an antibody that competes with the above-described monoclonal antibodies or antigen-binding portions thereof. In some embodiments, the invention relates to an antibody that competes with the above-described monoclonal antibodies or antigen-binding portions thereof.

在某些具體實施例,本發明係關於一種單株抗-人類CD52抗體或其抗原-結合部分,其中該抗體的重鏈及輕鏈分別包含SEQ ID NO: 272及273的胺基酸序列,且無信號序列。在某些具體實施例,本發明係關於一種單株抗-人類CD52抗體或其抗原-結合部分,其中該抗體的重鏈及輕鏈分別包含SEQ ID NO: 274及275的胺基酸序列,且無信號序列。在某些具體實施例,本發明係關於一種單株抗-人類CD52抗體或其抗原-結合部分,其中該抗體的重鏈及輕鏈分別包含SEQ ID NO: 276及278的胺基酸序列,且無信號序列。在某些具體實施例,本發明係關於一種單株抗-人類CD52抗體或其抗原-結合部分,其中該抗體的重鏈及輕鏈分別包含SEQ ID NO: 277及278的胺基酸序列,且無信號序列。在某些具體實施例,本發明係關於一種單株抗-人類CD52抗體或其抗原-結合部分,其中該抗體的重鏈及輕鏈分別包含SEQ ID NO: 279及280的胺基酸序列,且無信號序列。在某些具體實施例,本發明係關於一種單株抗-人類CD52抗體或其抗原-結合部分,其中該抗體的重鏈及輕鏈分別包含SEQ ID NO: 281及282的胺基酸序列,且無信號序列。In certain embodiments, the invention relates to a monoclonal anti-human CD52 antibody or antigen-binding portion thereof, wherein the heavy and light chains of the antibody comprise the amino acid sequences of SEQ ID NO: 272 and 273, respectively, And no signal sequence. In certain embodiments, the invention relates to a monoclonal anti-human CD52 antibody or antigen-binding portion thereof, wherein the heavy and light chains of the antibody comprise the amino acid sequences of SEQ ID NO: 274 and 275, respectively, And no signal sequence. In certain embodiments, the invention relates to a monoclonal anti-human CD52 antibody or antigen-binding portion thereof, wherein the heavy and light chains of the antibody comprise the amino acid sequences of SEQ ID NOs: 276 and 278, respectively, And no signal sequence. In certain embodiments, the invention relates to a monoclonal anti-human CD52 antibody or antigen-binding portion thereof, wherein the heavy and light chains of the antibody comprise the amino acid sequences of SEQ ID NOs: 277 and 278, respectively, And no signal sequence. In certain embodiments, the invention relates to a monoclonal anti-human CD52 antibody or antigen-binding portion thereof, wherein the heavy and light chains of the antibody comprise the amino acid sequences of SEQ ID NO: 279 and 280, respectively, And no signal sequence. In certain embodiments, the invention relates to a monoclonal anti-human CD52 antibody or antigen-binding portion thereof, wherein the heavy and light chains of the antibody comprise the amino acid sequences of SEQ ID NO: 281 and 282, respectively, And no signal sequence.

在一些具體實施例,本發明係關於一種單株抗-人類CD52抗體或其抗原-結合部分,其中該抗體的輕鏈包含由SEQ ID NOs: 102、138、145-148、153-157及164-168所組成族群選出的胺基酸序列。在某些具體實施例,本發明係關於一種單株抗-人類CD52抗體或其抗原-結合部分,其中該抗體的輕鏈包含由SEQ ID NOs: 273、275、278、280及282所組成族群選出的胺基酸序列,且無信號序列。在某些具體實施例,本發明係關於一種抗體的輕鏈或其抗原-結合部分,其包含由SEQ ID NOs: 102、138、145-148、153-157、164-168、273、275、278、280及282所組成族群選出的胺基酸序列,且無信號序列若存在。In some embodiments, the invention relates to a monoclonal anti-human CD52 antibody or antigen-binding portion thereof, wherein the light chain of the antibody comprises SEQ ID NOs: 102, 138, 145-148, 153-157, and 164 The amino acid sequence selected from the group consisting of -168. In certain embodiments, the invention relates to a monoclonal anti-human CD52 antibody or antigen-binding portion thereof, wherein the light chain of the antibody comprises a population consisting of SEQ ID NOs: 273, 275, 278, 280, and 282 The amino acid sequence was selected and there was no signal sequence. In certain embodiments, the invention relates to a light chain of an antibody or antigen-binding portion thereof, comprising SEQ ID NOs: 102, 138, 145-148, 153-157, 164-168, 273, 275, The amino acid sequence selected from the group consisting of 278, 280 and 282, and no signal sequence is present.

在一些具體實施例,本發明係關於一種單株抗-人類CD52抗體或其抗原-結合部分,其中該抗體的重鏈包含由SEQ ID NOs: 103、136、137、139-144、149-152及158-163所組成族群選出的胺基酸序列。在某些具體實施例,本發明係關於一種單株抗-人類CD52抗體或其抗原-結合部分,其中該抗體的重鏈包含由SEQ ID NOs: 272、274、276、277、279及281所組成族群選出的胺基酸序列,且無信號序列。在某些具體實施例,本發明係關於一種抗體重鏈或其部分,其包含由SEQ ID NOs: 103、136、137、139-144、149-152、158-163、272、274、276、277、279及281所組成族群選出的胺基酸序列,且無信號序列若存在。In some embodiments, the invention relates to a monoclonal anti-human CD52 antibody or antigen-binding portion thereof, wherein the heavy chain of the antibody comprises SEQ ID NOs: 103, 136, 137, 139-144, 149-152 And the amino acid sequence selected from the group consisting of 158-163. In certain embodiments, the invention relates to a monoclonal anti-human CD52 antibody or antigen-binding portion thereof, wherein the heavy chain of the antibody comprises SEQ ID NOs: 272, 274, 276, 277, 279, and 281 The amino acid sequence selected by the population is composed and has no signal sequence. In certain embodiments, the invention relates to an antibody heavy chain or a portion thereof comprising SEQ ID NOs: 103, 136, 137, 139-144, 149-152, 158-163, 272, 274, 276, The amino acid sequence selected from the group consisting of 277, 279 and 281, and no signal sequence is present.

在一些具體實施例,任何上述抗體可為IgG、IgM、IgA、IgD或IgE分子。在某些具體實施例,該IgG為IgG1、IgG2、IgG3、或IgG4。In some embodiments, any of the above antibodies can be an IgG, IgM, IgA, IgD or IgE molecule. In certain embodiments, the IgG is IgGl, IgG2, IgG3, or IgG4.

在一些具體實施例,任何上述抗原-結合部分可為單一鏈抗體、Fv、Fab、Fab'、F(ab')2、Fd、單一鏈Fv分子(scFv)、雙特定單一鏈Fv二聚體、雙鏈抗體、區域缺失抗體或單域抗體(dAb)。In some embodiments, any of the above antigen-binding moieties can be a single chain antibody, Fv, Fab, Fab', F(ab')2, Fd, single chain Fv molecule (scFv), bispecific single chain Fv dimer , a double-stranded antibody, a region deleted antibody, or a single domain antibody (dAb).

本發明亦關於任何上述抗體或抗原-結合部分,其中該抗體或抗原-結合部分消耗T或B淋巴細胞,或二者;與B淋巴細胞相較,較佳為消耗T淋巴細胞;增加TNF、IL-6、或MCP-1的循環血清含量;媒介CD52-表現細胞的抗體-依賴細胞介導性細胞毒性(ADCC);媒介CD52-表現細胞的補體依賴細胞毒性(CDC);及/或促進人類T及/或B細胞的細胞內發信號。The invention also relates to any of the above antibodies or antigen-binding portions, wherein the antibody or antigen-binding portion consumes T or B lymphocytes, or both; compared to B lymphocytes, preferably consumes T lymphocytes; increases TNF, Circulating serum levels of IL-6, or MCP-1; mediator CD52-antibody-dependent cell-mediated cytotoxicity (ADCC); mediator CD52-complementing cell-dependent cytotoxicity (CDC); and/or promotion Intracellular signaling of human T and/or B cells.

本發明進一步關於一種編碼任何上述抗體的重鏈或其抗原-結合部分,或是輕鏈或其抗原-結合部分之經分離核酸。在一些具體實施例,該經分離核酸包含由SEQ ID NOs: 283、285、287、288、290及292所組成族群選出的重鏈核苷酸序列,或是該核苷酸序列不具編碼信號胜肽的序列;由SEQ ID NOs: 284,286,289,291及293所組成族群選出的輕鏈核苷酸序列,或是該核苷酸序列不具編碼信號胜肽的序列;或是該重鏈核苷酸序列及該輕鏈核苷酸序列皆包含。在某些具體實施例,該經分離核酸所包含重鏈核苷酸序列與輕鏈核苷酸序列分別由SEQ ID NO: 283及SEQ ID NO: 284所組成族群選出,皆不具編碼信號胜肽的序列;分別由SEQ ID NO: 285及SEQ ID NO: 286所組成族群選出,皆不具編碼信號胜肽的序列;分別由SEQ ID NO: 287及SEQ ID NO: 289所組成族群選出,皆不具編碼信號胜肽的序列;分別由SEQ ID NO: 288及SEQ ID NO: 289所組成族群選出,皆不具編碼信號胜肽的序列;分別由SEQ ID NO: 290及SEQ ID NO: 291所組成族群選出,皆不具編碼信號胜肽的序列;及分別由SEQ ID NO: 292及SEQ ID NO: 293所組成族群選出,皆不具編碼信號胜肽的序列。The invention further relates to an isolated nucleic acid encoding a heavy chain of any of the above antibodies, or an antigen-binding portion thereof, or a light chain or antigen-binding portion thereof. In some embodiments, the isolated nucleic acid comprises a heavy chain nucleotide sequence selected from the group consisting of SEQ ID NOs: 283, 285, 287, 288, 290, and 292, or the nucleotide sequence does not have a coding signal. a sequence of a peptide; a light chain nucleotide sequence selected from the group consisting of SEQ ID NOs: 284, 286, 289, 291, and 293, or a sequence in which the nucleotide sequence does not encode a signal peptide; or the heavy chain nucleotide sequence and the The light chain nucleotide sequence is included. In some embodiments, the isolated nucleic acid comprises a heavy chain nucleotide sequence and a light chain nucleotide sequence selected from the group consisting of SEQ ID NO: 283 and SEQ ID NO: 284, respectively, without a coding signal peptide Sequences; selected from the group consisting of SEQ ID NO: 285 and SEQ ID NO: 286, respectively, without the sequence encoding the signal peptide; selected from the group consisting of SEQ ID NO: 287 and SEQ ID NO: 289, respectively a sequence encoding a signal peptide; selected from the group consisting of SEQ ID NO: 288 and SEQ ID NO: 289, respectively, without a sequence encoding a signal peptide; groups consisting of SEQ ID NO: 290 and SEQ ID NO: 291, respectively The sequences which are selected to have no coding signal peptide are selected; and the sequences consisting of SEQ ID NO: 292 and SEQ ID NO: 293, respectively, have no sequence encoding the signal peptide.

本發明亦關於使用包含重鏈核苷酸序列的經分離核酸及包含輕鏈核苷酸序列的經分離核酸以製造治療需要此種治療的病人之藥物,其中該重鏈核苷酸序列及該輕鏈核苷酸序列係由分別由SEQ ID NO: 283及SEQ ID NO: 284所組成族群選出,皆不具編碼信號胜肽的序列;分別由SEQ ID NO: 285及SEQ ID NO: 286所組成族群選出,皆不具編碼信號胜肽的序列;分別由SEQ ID NO: 287及SEQ ID NO: 289所組成族群選出,皆不具編碼信號胜肽的序列;分別由SEQ ID NO: 288及SEQ ID NO: 289所組成族群選出,皆不具編碼信號胜肽的序列;分別由SEQ ID NO: 290及SEQ ID NO: 291所組成族群選出,皆不具編碼信號胜肽的序列;及分別由SEQ ID NO: 292及SEQ ID NO: 293所組成族群選出,皆不具編碼信號胜肽的序列。The invention also relates to the use of an isolated nucleic acid comprising a heavy chain nucleotide sequence and an isolated nucleic acid comprising a light chain nucleotide sequence for the manufacture of a medicament for treating a patient in need of such treatment, wherein the heavy chain nucleotide sequence and The light chain nucleotide sequence is selected from the group consisting of SEQ ID NO: 283 and SEQ ID NO: 284, respectively, and has no coding signal peptide; it consists of SEQ ID NO: 285 and SEQ ID NO: 286, respectively. The population is selected, and the sequence encoding the signal peptide is not selected; the sequences consisting of SEQ ID NO: 287 and SEQ ID NO: 289, respectively, have no sequence encoding the signal peptide; SEQ ID NO: 288 and SEQ ID NO, respectively : 289 selected populations, none of which have a sequence encoding a peptide; selected from the group consisting of SEQ ID NO: 290 and SEQ ID NO: 291, respectively, without a sequence encoding a signal peptide; and by SEQ ID NO: The group consisting of 292 and SEQ ID NO: 293 was selected and did not have a sequence encoding a signal peptide.

本發明亦關於一種重組載體,其包含(1)編碼任何上述抗體的重鏈或其抗原-結合部分的核酸序列,(2)編碼任何上述抗體的輕鏈或其抗原-結合部分的核酸序列,或(3)二者。本發明進一步關於一種宿主細胞,其包含:編碼任何上述抗體的重鏈或其抗原-結合部分的第一核酸序列,該第一核酸序列操作地鏈結至表現控制因子;及編碼該抗體的輕鏈或其抗原-結合部分的第二核酸序列,該第二核酸序列操作地鏈結至表現控制因子。本發明係關於一種抗-人類CD52抗體或其抗原-結合部分的製造方法,其包含維持該宿主細胞在適合該抗體或部分表現的條件下,及亦關於該方法,其進一步包含分離該抗體或部分的步驟。The present invention also relates to a recombinant vector comprising (1) a nucleic acid sequence encoding a heavy chain of any of the above antibodies or an antigen-binding portion thereof, and (2) a nucleic acid sequence encoding a light chain of any of the above antibodies or an antigen-binding portion thereof, Or (3) both. The invention further relates to a host cell comprising: a first nucleic acid sequence encoding a heavy chain of any of the above antibodies, or an antigen-binding portion thereof, operably linked to a expression control factor; and a light encoding the antibody A second nucleic acid sequence of a strand or antigen-binding portion thereof, the second nucleic acid sequence operably linked to a performance control factor. The present invention relates to a method for producing an anti-human CD52 antibody or antigen-binding portion thereof, comprising maintaining the host cell under conditions suitable for the antibody or partial expression, and also relating to the method, further comprising isolating the antibody or Part of the steps.

本發明係關於一種組合物,其包含根據申請專利範圍第1-24項中任一項的單株抗體或抗原-結合部分及醫藥可接受媒劑或載體。The present invention relates to a composition comprising a monoclonal antibody or antigen-binding portion according to any one of claims 1 to 24 and a pharmaceutically acceptable vehicle or carrier.

在一些具體實施例,本發明係關於一種需要此種治療的病人之治療方法,其包含投藥有效量的任何上述抗體或抗原-結合部分,或是上述組合物予病人。在某些具體實施例,該病人正接受移植。In some embodiments, the invention is directed to a method of treating a patient in need of such treatment comprising administering an effective amount of any of the above antibodies or antigen-binding moieties, or the above composition to a patient. In some embodiments, the patient is undergoing a transplant.

在一些具體實施例,本發明係關於一種需要自體免疫疾病治療的病人之治療方法,其包含投藥有效量的任何上述抗體或抗原-結合部分,或是上述組合物予病人。在某些具體實施例,該自體免疫疾病為,例如,多發性硬化症、風濕性關節炎、或系統性紅斑狼瘡。In some embodiments, the invention is directed to a method of treating a patient in need of treatment with an autoimmune disease comprising administering an effective amount of any of the above antibodies or antigen-binding moieties, or the above composition to a patient. In certain embodiments, the autoimmune disease is, for example, multiple sclerosis, rheumatoid arthritis, or systemic lupus erythematosus.

在一些具體實施例,本發明係關於一種需要癌症治療的病人之治療方法,其包含投藥有效量的任何上述抗體或抗原-結合部分,或是上述組合物予病人。在某些具體實施例,該癌症為,例如,具巨大腫瘤的非-何杰金氏淋巴瘤;B-細胞慢性淋巴性白血病;T細胞惡性腫瘤,其中與B細胞相較,該抗體或部分較佳為消耗T細胞;或是實體腫瘤。In some embodiments, the invention relates to a method of treating a patient in need of cancer treatment comprising administering an effective amount of any of the above antibodies or antigen-binding moieties, or the above composition to a patient. In certain embodiments, the cancer is, for example, a non-Hodgkin's lymphoma with a large tumor; a B-cell chronic lymphocytic leukemia; a T cell malignancy, wherein the antibody or portion is compared to a B cell Preferably, the T cells are consumed; or a solid tumor.

在一些具體實施例,任何上述治療方法進一步包含投藥嗜中性球或NK細胞刺激劑予病人。在某些具體實施例,該藥劑係為G-CSF或GM-CSF。在一些具體實施例,任何上述治療方法進一步包含投藥T調節細胞刺激劑予病人。在某些具體實施例,該藥劑係為雷帕黴素。In some embodiments, any of the above methods of treatment further comprises administering a neutrophil or NK cell stimulating agent to the patient. In certain embodiments, the agent is G-CSF or GM-CSF. In some embodiments, any of the above methods of treatment further comprises administering a T-modulating cell stimulating agent to the patient. In certain embodiments, the agent is rapamycin.

在一些具體實施例,本發明係關於一種有需要的病人中血管新生抑制方法,其包含投藥有效量的任何上述抗體或抗原-結合部分予病人。在某些具體實施例,該病人具實體腫瘤。在某些具體實施例,該病人具血管新生。在某些具體實施例,該血管新生係在眼睛。In some embodiments, the invention relates to a method of inhibiting angiogenesis in a patient in need thereof, comprising administering an effective amount of any of the above antibodies or antigen-binding moieties to a patient. In some embodiments, the patient has a solid tumor. In some embodiments, the patient has angiogenesis. In certain embodiments, the angiogenesis is in the eye.

本發明亦關於使用任何上述抗體或抗原-結合部分以製造治療有需要病人中自體免疫疾病之藥物。更進一步,本發明係關於使用任何上述抗體或抗原-結合部分以製造治療有需要病人中癌症之藥物。本發明係關於使用任何上述抗體或抗原-結合部分以製造治療有需要移植的病人之藥物。本發明係關於使用任何上述抗體或抗原-結合部分以製造治療有需要病人中血管新生之藥物。The invention also relates to the use of any of the above antibodies or antigen-binding moieties to produce a medicament for the treatment of an autoimmune disease in a patient in need thereof. Still further, the present invention relates to the use of any of the above antibodies or antigen-binding moieties to produce a medicament for treating cancer in a patient in need thereof. The present invention relates to the use of any of the above antibodies or antigen-binding moieties to manufacture a medicament for treating a patient in need of transplantation. The present invention relates to the use of any of the above antibodies or antigen-binding moieties to produce a medicament for the treatment of angiogenesis in a patient in need thereof.

本發明亦關於使用任何上述抗體或抗原-結合部分做為藥物。The invention also relates to the use of any of the above antibodies or antigen-binding moieties as a medicament.

CD52為一種醣化,GPI錨定細胞表面富含蛋白(約5 x 105個抗體結合部位每個細胞),其存在於至少95%的所有人類週邊血液淋巴細胞及單核細胞/巨噬細胞(Hale G,等「The CAMPATH-1 antigen(CD52),」Tissue Antigens,35:178-327(1990)),但是不存在於造血幹細胞。本發明係關於具結合至或選擇性結合至人類CD52或其部份的結合專一性(例如,抗原決定區專一性)免疫球蛋白(抗-CD52)。這些免疫球蛋白特定地結合至CD52,及不會特定地結合至非-CD52分子。在抗-CD52免疫球蛋白及CD52之間的特定結合可由,例如,使用流式細胞計數法測量免疫球蛋白結合至CD52+細胞的EC50而決定。特定結合可由例如0.5-10微克/毫升的EC50範圍所顯示。此處所敘述免疫球蛋白可具所有或部份人類CD52的結合專一性,其中人類CD52為經分離的及/或重組人類CD52,或是於表現人類CD52的細胞表面。此外,免疫球蛋白可具一或更多型式的人類CD52(例如,經醣化人類CD52;去-醣化人類CD52;非-醣化人類CD52;及對偶基因變異體)的結合專一性。在一個具體實施例,免疫球蛋白具自然發生,內源型或野生型人類CD52的結合專一性。野生型人類CD52的胺基酸序列說明於第4圖(SEQ ID NO: 104)。CD52 is a glycosylation, and GPI anchors cell surface-rich proteins (about 5 x 10 5 antibody binding sites per cell) present in at least 95% of all human peripheral blood lymphocytes and monocytes/macrophages ( Hale G, et al., "The CAMPATH-1 antigen (CD52)," Tissue Antigens , 35: 178-327 (1990)), but not in hematopoietic stem cells. The present invention relates to immunospecific globulin (anti-CD52) having binding specificity (e.g., antigenic epitope specificity) that binds to or selectively binds to human CD52 or a portion thereof. These immunoglobulins specifically bind to CD52 and do not specifically bind to non-CD52 molecules. -CD52 between the anti-CD52 immunoglobulin and the specific binding by, e.g., using flow cytometry measurements of immune globulin to bind CD52 + EC 50 cells is determined. Specific binding may range e.g. EC 50 0.5-10 [mu] g / ml displayed. The immunoglobulins described herein may have the binding specificity of all or part of human CD52, which is an isolated and/or recombinant human CD52, or a cell surface that exhibits human CD52. In addition, immunoglobulins may have one or more types of human CD52 (eg, glycosylated human CD52; de-glycosylated human CD52; non-glycosylated human CD52; and dual gene variants). In a specific embodiment, the immunoglobulin has a naturally occurring, endogenous or wild type human CD52 binding specificity. The amino acid sequence of wild type human CD52 is illustrated in Figure 4 (SEQ ID NO: 104).

此處所敘述免疫球蛋白可使用已知技術純化或分離。「純化」或"分離"的免疫球蛋白已自其起源(例如,細胞上層清液;於混合物中,例如於抗體庫的免疫球蛋白的混合物中)分子(例如,肽)分開,及包含由此處所敘述方法或其他合適方法所得到的免疫球蛋白。經分離免疫球蛋白包含大體上純的(實質上純的)免疫球蛋白,及由化學合成,重組技術及其組合所製造的免疫球蛋白。The immunoglobulins described herein can be purified or isolated using known techniques. "purified" or "isolated" immunoglobulins have been separated from their origin ( eg, cell supernatant; in a mixture, such as a mixture of immunoglobulins in an antibody library) molecules (eg, peptides), and Immunoglobulins obtained by the methods described herein or other suitable methods. Isolated immunoglobulins comprise substantially pure (substantially pure) immunoglobulins, and immunoglobulins produced by chemical synthesis, recombinant techniques, and combinations thereof.

更特定言之,本發明係關於抗-人類CD52免疫球蛋白、免疫球蛋白的抗原-結合片段(亦即,部分)、免疫球蛋白的輕鏈、免疫球蛋白的重鏈、及這些輕鏈或重鏈的片段。本發明亦關於成熟免疫球蛋白或其鏈,例如醣化免疫球蛋白。本發明亦關於成熟或前軀體免疫球蛋白(蛋白)。本發明亦關於編碼這些不成熟或成熟蛋白的核酸分子(例如,載體),關於包含此種核酸的載體及宿主細胞,關於不成熟及成熟蛋白的製造方法及關於免疫球蛋白的使用方法。More particularly, the present invention relates to anti-human CD52 immunoglobulins, antigen-binding fragments (i.e., portions) of immunoglobulins, light chains of immunoglobulins, heavy chains of immunoglobulins, and these light chains. Or a fragment of a heavy chain. The invention also relates to mature immunoglobulins or chains thereof, such as glycated immunoglobulins. The invention also relates to mature or precursor immunoglobulins (proteins). The invention also relates to nucleic acid molecules ( e.g. , vectors) encoding such immature or mature proteins, to vectors and host cells comprising such nucleic acids, to methods of making immature and mature proteins, and to methods of using immunoglobulins.

本發明免疫球蛋白可用於治療需要的個體(例如,人類病人)以消耗個體的淋巴細胞及依所需其他CD52+細胞。當用於此處時,」淋巴細胞消耗」為一種藉由減少循環淋巴細胞族群(例如,T細胞及/或B細胞)而造成淋巴細胞減少的免疫抑制形式。本發明免疫球蛋白亦可用於抑制血管新生,如於下文進一步敘述。The immunoglobulins of the invention can be used to treat a subject in need (e.g., a human patient) to consume lymphocytes from the individual and other CD52+ cells as desired. When used herein, "lymphocyte depletion" is an immunosuppressive form that causes lymphopenia by reducing circulating lymphocyte populations (e.g., T cells and/or B cells). The immunoglobulins of the invention may also be used to inhibit angiogenesis as further described below.

自然發生的免疫球蛋白具共同核心結構,其中兩個相同輕鏈(約24 kD)及兩個相同重鏈(約55或70 kD)形成一個四聚物。每一個鏈的胺基-端部份係已知為變異(V)區及可與每一個鏈的其餘部分更守恆的恆定(C)區分別。在輕鏈變異區(亦稱為VL域)內為已知為J區域的C-端部分。在重鏈變異區(亦稱為VH域)內,除了J區域還有D區域。在免疫球蛋白的大部分胺基酸序列變異侷限為在V區域的三個個別位置,其稱為高變異區或互補決定區段(CDR),其係直接涉及抗原結合。自胺基-端開始,這些區段係分別命名為CDR1、CDR2及CDR3。這些CDR係藉由更守恆的骨架區(FR)固定於所在處。自胺基-端開始,這些區段係分別命名為FR1、FR2、FR3及FR4。CDR及FR區段的位置及編號系統已由Kabat(Kabat,E.A.,et al.,Sequences of Proteins of Immunological Interest,Fifth Edition,U.S. Department of Health and Human Services,U.S. Government Printing Office(1991),Chothia & Lesk,Canonical Structures for the Hypervariable Regions of Immunoglobulins,J. Mol. Biol.,196,901-917(1987),及IMGT編號系統(The International ImMunoGeneTics Iinformation Ssystem,Lefranc,M.-P.,The Immunologist 7,132-136(1999)定義。可執行視覺檢查及序列分析以辨識CDR邊際。對於本發明,CDR係藉由使用Kabat系統及IMGT系統而定義;亦即,當由該兩個系統定義的CDR未完全重疊,我們包含來自由該兩個系統所定義序列的殘基。Naturally occurring immunoglobulins have a common core structure in which two identical light chains (about 24 kD) and two identical heavy chains (about 55 or 70 kD) form a tetramer. The amine-terminal portion of each chain is known as the variant (V) region and a constant (C) region that is more conserved with the remainder of each chain, respectively. The light chain variable region (also referred to as V L domain) is known as the C- terminal portion of the J region. Within the heavy chain variant region (also known as the VH domain), there is a D region in addition to the J region. Most amino acid sequence variations in immunoglobulins are limited to three individual positions in the V region, which are referred to as high variant regions or complementarity determining segments (CDRs), which are directly involved in antigen binding. Starting from the amino-terminus, these segments are designated CDR1, CDR2 and CDR3, respectively. These CDRs are fixed at their location by a more conserved framework region (FR). Starting from the amino-terminus, these segments are designated FR1, FR2, FR3 and FR4, respectively. CDR and FR and the position of the section by the Kabat et al numbering system (Kabat, EA, et al. , Sequences of Proteins of Immunological Interest, Fifth Edition, US Department of Health and Human Services, US Government Printing Office (1991), Chothia & Lesk, Canonical Structures for the Hypervariable Regions of Immunoglobulins , J. Mol. Biol., 196, 901-917 (1987), and IMGT Numbering System (The International ImMunoGeneTics Iinformation Ssystem , Lefranc, M.-P., The Immunologist 7 , 132-136 (1999). Visual inspection and sequence analysis can be performed to identify the CDR margins. For the purposes of the present invention, CDRs are defined by the use of the Kabat system and the IMGT system; that is, when the CDRs defined by the two systems do not completely overlap, we contain residues from the sequences defined by the two systems.

依據重鏈的同種型而定,人類免疫球蛋白可分為分為類及亞類,類包含IgG、IgM、IgA、IgD及IgE,其中重鏈分別為gamma(γ)、mu(μ)、alpha(α)、delta(δ)或epsilon(ε)型式。亞類包含IgG1、IgG2、IgG3、IgG4、IgA1及IgA2,其中重鏈分別為γ1、γ2、γ3、γ4、α1及α2型式。所選擇類或亞類的人類免疫球蛋白分子可包含kappa(κ)或lambda(λ)輕鏈。參考例如Cellular and Molecular Immunology,Wonsiewicz,M.J.,Ed.,Chapter 45,pp. 41-50,W. B. Saunders Co.,Philadelphia,PA 91991);Nisonoff,A.,Introduction to Molecular Immunology,2nd Ed.,Chapter 4,pp. 45-65,Sinauer Associates,Inc.,Sunderland,MA(1984)。According to the isotype of heavy chain, human immunoglobulin can be divided into classes and subclasses, including IgG, IgM, IgA, IgD and IgE, wherein the heavy chains are gamma (γ), mu (μ), Alpha (α), delta (δ) or epsilon (ε) type. The subclasses include IgG1, IgG2, IgG3, IgG4, IgA1, and IgA2, wherein the heavy chains are γ1, γ2, γ3, γ4, α1, and α2, respectively. The human immunoglobulin molecule of the selected class or subclass may comprise a kappa (κ) or lambda (λ) light chain. References include, for example, Cellular and Molecular Immunology , Wonsiewicz, MJ, Ed., Chapter 45, pp. 41-50, WB Saunders Co., Philadelphia, PA 91991); Nisonoff, A., Introduction to Molecular Immunology , 2 nd Ed., Chapter 4, pp. 45-65, Sinauer Associates, Inc., Sunderland, MA (1984).

當用於此處時,名稱「免疫球蛋白」及「抗體」,其係交互使用來表示整體抗體及抗原-結合片段(亦即,"抗原-結合部份"-除非另外指出,否則於此處該兩個名稱係互換使用)。抗體的抗原-結合部份可為例如單鏈抗體、Fv片段、Fab片段、Fab'片段、F(ab')2片段、Fd片段、單鏈Fv分子(scFv)、雙特定單鏈Fv二聚體(PCT/US92/09665)、雙鏈抗體、區域缺失抗體及單域抗體(dAbs)的格式。參考例如,Nature Biotechnology 22(9):1161-1165(2004))。亦在本發明範圍內的是包含VH及/或VL的抗原-結合分子。在VH的情況,分子亦可包含一或更多CH1、鉸接處、CH2及CH3區域。意欲包含此種單鏈抗體於"抗原-結合部份"的名稱抗體內。As used herein, the terms "immunoglobulin" and "antibody" are used interchangeably to refer to whole antibodies and antigen-binding fragments (ie, "antigen-binding portions" - unless otherwise indicated The two names are used interchangeably). The antigen-binding portion of the antibody may be, for example, a single chain antibody, an Fv fragment, a Fab fragment, a Fab' fragment, an F(ab') 2 fragment, an Fd fragment, a single chain Fv molecule (scFv), a bispecific single chain Fv dimerization. Format of PCT/US92/09665, double-stranded antibodies, region-deficient antibodies, and single-domain antibodies (dAbs). For example, Nature Biotechnology 22(9): 1161-1165 (2004)). Also within the scope of the invention are antigen-binding molecules comprising VH and/or VL. In the case of VH, the molecule may also contain one or more CH1, hinge, CH2 and CH3 regions. It is intended to include such a single chain antibody within the name antibody of the "antigen-binding portion".

抗體部份或片段可由酶催化裂解或由重組技術製造。例如,可使用木瓜酵素或胃蛋白酶裂解以分別產生Fab或F(ab')2片段。亦可使用已引入一或更多中止密碼子於天然終止部位上游的抗體基因以各種截短樣式製造抗體。例如,編碼F(ab')2片段的重鏈之重組構成物可設計為包含編碼重鏈的CH1域及鉸鏈區的DNA序列。較佳抗原-結合片段具野生型人類CD52的結合專一性。Antibody fractions or fragments can be produced by enzymatic cleavage or by recombinant techniques. For example, papain or pepsin cleavage can be used to generate Fab or F(ab') 2 fragments, respectively. Antibodies can also be made in various truncated styles using antibody genes that have introduced one or more stop codons upstream of the natural termination site. For example, a recombinant construct encoding a heavy chain F (ab ') 2 fragment can be designed to CH 1 domain and hinge region of the heavy chain encoding DNA sequences. Preferred antigen-binding fragments have the specificity of binding to wild-type human CD52.

在另一方面,本發明提供一種抗體或此處所敘述部份的變化,其中該變化物特定地結合至人類CD52,但與參考抗體或其部份差異為1、2、3、4、5、6、7、8、9或10個胺基酸取代(例如,在CDR區域、FR區域、或侷限區域)。例如,變化抗體為於重鏈、重鏈變異區、輕鏈、或輕鏈變異區至少90%、至少91%、至少93%、至少95%、至少97%或至少99%相同於參考抗體。In another aspect, the invention provides a change in an antibody or a portion described herein, wherein the variant specifically binds to human CD52, but differs from the reference antibody or portion thereof by 1, 2, 3, 4, 5, 6, 7, 8, 9 or 10 amino acid substitutions (eg, in the CDR regions, FR regions, or confined regions). For example, a variant antibody is at least 90%, at least 91%, at least 93%, at least 95%, at least 97%, or at least 99% identical to a reference antibody in the heavy chain, heavy chain variant region, light chain, or light chain variant region.

多肽的序列相似性或同源性,其亦稱為序列同源性,典型上係使用序列分析軟體測量。蛋白分析軟體使用指派為各種取代、消除及其他修飾(包含保守型胺基酸取代)的相似性度量。來符合類似序列。舉例而言,GCG包含諸如"Gap"及"Bestfit"的程式,其可使用預設參數以決定緊密相關多肽(例如得自不同有機物種的同系多肽)之間或是野生型蛋白及其突變蛋白之間的序列同源性或序列一致性。參看例如GCG 6.1版。亦可使用利用預設或建議參數的FASTA(GCG 6.1版的程式)比較多肽序列。FASTA(例如,FASTA2及FASTA3)提供欲排列序列及搜尋序列之間的最佳重疊區域的排列及百分率序一致源性(Pearson,Methods EnzymoL. 183:63-98(1990);Pearson,Methods MoL. Biol.132:185-219(2000))。當比較本發明序列與包含大量來自不同有機體的序列之資料庫時,另一種較佳演算法為電腦程式BLAST,特別是blastp或tblastn,其係使用預設參數。參看例如Altschul等,J. Mol. Biol. 215:403-410(1990);Altschul et al.,Nucleic Acids Res. 25:3389-402(1997);此處併入做為參考。Sequence similarity or homology of a polypeptide, also referred to as sequence homology, is typically measured using sequence analysis software. Protein analysis software uses a measure of similarity assigned to various substitutions, eliminations, and other modifications, including conservative amino acid substitutions. To conform to a similar sequence. For example, GCG includes programs such as "Gap" and "Bestfit" that can use preset parameters to determine closely related polypeptides (eg, homologous polypeptides from different organic species) or between wild-type proteins and their mutant proteins. Sequence homology or sequence identity between. See, for example, GCG version 6.1. The polypeptide sequence can also be compared using FASTA (program of GCG version 6.1) using preset or suggested parameters. FASTA (e.g., FASTA2 and FASTA3) provides alignment and percent order identity of the optimal overlap region between the sequence to be searched and the search sequence (Pearson, Methods Enzymo L. 183: 63-98 (1990); Pearson, Methods MoL. Biol. 132: 185-219 (2000)). Another preferred algorithm when comparing the sequences of the invention to a library containing a large number of sequences from different organisms is the computer program BLAST, in particular blastp or tblastn, which uses preset parameters. See, for example, Altschul et al, J. Mol. Biol. 215: 403-410 (1990); Altschul et al., Nucleic Acids Res. 25: 3389-402 (1997); incorporated herein by reference.

根據本發明,可進行的一種型式的胺基酸取代為變更抗體中一或更多半胱氨酸(其可為化學反應性的)為另一種殘基物(例如而不限於丙胺酸或絲胺酸)。在一個具體實施例,存在非-正則半胱氨酸的取代反應。取代反應可在抗體的CDR或變異區的骨架區中或在恆定區中進行。在一些具體實施例,半胱氨酸為正則的。可進行的另一種型式的胺基酸取代為移除抗體中潛在蛋白酵素部位。此種部位可發生於抗體的CDR或變異區的骨架區中或於恆定區中。半胱氨酸殘基物的取代反應及蛋白酵素部位的移除會減少抗體產物中不均勻性的風險及於是增加其均勻性。另一種型式的胺基酸取代為藉由變更殘基的一個或二者而消除天門冬胺酸-甘胺酸對,其形成潛在去醯胺化部位。在本發明另一方面,可使用敘述於例如PCT公開WO98/52976及WO00/34317的技術去免疫型抗體以減少其致免疫性。In accordance with the present invention, one type of amino acid substitution that can be made is to alter one or more cysteines (which may be chemically reactive) in the antibody to another residue (eg, without limitation, alanine or silk) Amino acid). In a specific embodiment, there is a substitution reaction of non-regular cysteine. The substitution reaction can be carried out in the framework region of the CDR or variant region of the antibody or in the constant region. In some embodiments, the cysteine is regular. Another type of amino acid substitution that can be made is to remove potential protein enzyme sites in the antibody. Such a site may occur in the framework region of the CDR or variant region of the antibody or in the constant region. The substitution reaction of the cysteine residue and the removal of the proteinase site reduce the risk of heterogeneity in the antibody product and thus increase its uniformity. Another type of amino acid substitution is to eliminate the aspartic acid-glycine pair by altering one or both of the residues, which form a potential deamination site. In another aspect of the invention, deimmunized antibodies can be used to reduce their immunogenicity using techniques such as those described in PCT Publication Nos. WO 98/52976 and WO 00/34317.

可在根據本發明變化中的一個進行的另一種型式的胺基酸取代為保守型胺基酸取代反應。"保守型胺基酸取代反應"為一種胺基酸殘基由具類似化學性質(例如,電荷或疏水性)的側鏈R基的另一個胺基酸殘基所取代的取代反應。一般,保守型胺基酸取代反應大體上不會變更蛋白的功能性質。在二或更多胺基酸序列因保守型取代反應彼此不同的情況,可向上調整百分率序列一致性或相似度以修正取代反應的保守本質。進行此調整的方式為熟知該技藝者所已知。參看例如Pearson,Methods Mol. Biol. 243:307-31(1994)。Another type of amino acid substitution that can be carried out in accordance with one of the variations of the present invention is a conservative amino acid substitution reaction. A "conservative amino acid substitution reaction" is a substitution reaction in which an amino acid residue is substituted with another amino acid residue of a side chain R group having a similar chemical property (for example, charge or hydrophobicity). In general, conservative amino acid substitution reactions do not substantially alter the functional properties of the protein. In the case where two or more amino acid sequences differ from each other due to the conservative substitution reaction, the percent sequence identity or similarity can be adjusted upward to correct the conservative nature of the substitution reaction. The manner in which this adjustment is made is known to those skilled in the art. See, for example, Pearson, Methods Mol. Biol. 243:307-31 (1994).

具類似化學性質側鏈的胺基酸實例包含1)脂族側鏈:甘胺酸、丙胺酸、纈胺酸、白胺酸白胺酸、及異白胺酸白胺酸;2)脂族-羥基側鏈:絲氨酸及蘇胺酸;3)含醯胺側鏈:天門冬胺酸及麩醯胺;4)芳香族側鏈:苯丙胺酸丙胺酸、酪氨酸、及色氨酸;5)鹼式側鏈:離胺酸、精胺酸、及組氨酸;6)酸式側鏈:門冬氨酸及谷氨酸;及7)含硫側鏈:半胱氨酸及蛋氨酸。較佳保守型胺基酸取代反應組為:纈胺酸-白胺酸白胺酸-異白胺酸白胺酸、苯丙胺酸丙胺酸-酪氨酸、離胺酸-精胺酸、丙胺酸-纈胺酸、麩胺酸-天冬氨酸、及天門冬胺酸-麩醯胺。或者是,保守型置換反應為在揭示於Science 256:1443-45(1992)的PAM250對數似矩陣中具正值的任何變更(Gonnet等)。"中度保守型"置換為在PAM250對數似矩陣具非負值的任何變更。Examples of amino acids having similar chemical side chains include 1) aliphatic side chains: glycine, alanine, valine, leucine, and isoleucine; 2) aliphatic -hydroxy side chain: serine and threonine; 3) guanamine containing side chain: aspartic acid and glutamine; 4) aromatic side chain: phenylalanine alanine, tyrosine, and tryptophan; Basic side chain: lysine, arginine, and histidine; 6) acid side chain: aspartic acid and glutamic acid; and 7) sulfur-containing side chain: cysteine and methionine. The preferred conservative amino acid substitution reaction group is: valine acid-leucine leucine-isoleucine leucine, phenylalanine-alanine-tyrosine, lysine-arginine, alanine - Proline, glutamic acid - aspartic acid, and aspartic acid - branamide. Alternatively, the conservative substitution reaction is any change in the positive value of the PAM250 log-like matrix disclosed in Science 256:1443-45 (1992) (Gonnet et al). The "moderately conservative" substitution is any change that has a non-negative value on the PAM250 log-like matrix.

在某些具體實施例,對本發明抗體或抗原-結合部分的胺基酸取代反應為:(1)減少對蛋白質水解的敏感性,(2)減少對氧化反應的敏感性,(3)改變對形成蛋白複合物的結合親合力,例如,以增強抗體的ADCC及CDC活性,(4)賦予或修飾此種類似物的其他物理化學或功能性質,但仍保留至人類CD52的特定結合,(5)移除C-端離胺酸,及(6)增加或移除醣化部位。In certain embodiments, the amino acid substitution reaction of an antibody or antigen-binding portion of the invention is: (1) reduced sensitivity to proteolysis, (2) reduced sensitivity to oxidation, and (3) altered pair Forming the binding affinity of the protein complex, for example, to enhance the ADCC and CDC activity of the antibody, (4) imparting or modifying other physicochemical or functional properties of the analog, but retaining the specific binding to human CD52, (5) Remove the C-terminus from the amine acid, and (6) increase or remove the glycation site.

在一方面,本發明提供一種為本發明抗體的重或輕鏈的新型及新穎多肽,或是其為重或輕鏈的含變異區部分。此種多肽為有用的因為其可與相對(輕或重)抗體鏈組合以形成CD52-結合分子。In one aspect, the invention provides a novel and novel polypeptide of the heavy or light chain of an antibody of the invention, or a portion of a variant comprising a heavy or light chain. Such polypeptides are useful because they can be combined with relatively (light or heavy) antibody chains to form CD52-binding molecules.

人類化免疫球蛋白Human immunoglobulin

此處所敘述為包含新穎老鼠抗-人類CD52抗體CDRs的人類化免疫球蛋白。在一個具體實施例,人類化免疫球蛋白包含具與抗-CD52抗體其他人類化類型(例如,Campath)的胺基酸序列不同的CDR胺基酸序列之人類化輕鏈及人類化重鏈。Described herein are humanized immunoglobulins comprising novel mouse anti-human CD52 antibody CDRs. In a specific embodiment, the human immunoglobulin comprises other humanized types with anti-CD52 antibodies ( eg, Campath Humanized light chains and humanized heavy chains of CDR amino acid sequences differing in amino acid sequence.

名稱「人類化免疫球蛋白」當用於此處時係表示一種免疫球蛋白,其包含非-人類來源的抗-CD52抗體,此處亦稱為授予體抗體(例如,小鼠抗-CD52抗體),的一或更多輕鏈CDR(CDR1、CDR2及CDR3)及一或更多重鏈CDR(CDR1、CDR2及CDR3)的鏈,及至少一部份人類來源的免疫球蛋白(例如,得自人類來源的輕及/或重鏈的骨架區,或骨架區與恆定區,例如具或不具骨架變更的CDR-移植抗體)。本發明人類化免疫球蛋白包含與存在於Campath的至少一個CDR(例如,來自相對應CDR)不同的至少一個CDR。參看:例如Cabilly,美國專利第4,816,567號;Cabilly等,歐洲專利第0,125,023 B1號;Boss等,美國專利第4,816,397號;Boss等,歐洲專利第0,120,694 B1號;Neuberger,M.S.等,WO 86/01533;Neuberger,M.S.等,歐洲專利第0,194,276 B1號;Winter美國專利第5,225,539號;Winter歐洲專利第0,239,400 B1號;Padlan,E.A.等,歐洲專利申請案第0,519,596 A1號。關於單一鏈抗體,亦參看:Ladner等,美國專利第4,946,778號;Huston美國專利第5,476,786號;及Bird,R.E.等, Science,242: 423-426(1988))。在一些具體實施例,人類化免疫球蛋白為一種去免疫型抗體。參看例如Carr等,美國專利第7,264,806號,其關於已修飾以減少潛在T-細胞抗原決定區的數目之去免疫型免疫球蛋白,由此減少免疫球蛋白在投藥至人類時引出免疫反應的傾向。The term "humanized immunoglobulin" as used herein refers to an immunoglobulin comprising an anti-CD52 antibody of non-human origin, also referred to herein as a donor antibody ( eg, a mouse anti-CD52 antibody). a chain of one or more light chain CDRs (CDR1, CDR2 and CDR3) and one or more heavy chain CDRs (CDR1, CDR2 and CDR3), and at least a portion of a human-derived immunoglobulin ( eg, A framework region of light and/or heavy chains of human origin, or a framework region and a constant region, such as a CDR-grafted antibody with or without a framework change). The humanized immunoglobulin of the present invention is contained and present in Campath At least one CDR ( eg, from a corresponding CDR) differs from at least one CDR. See, for example, Cabilly et al ., U.S. Patent No. 4,816,567; Cabilly et al., European Patent No. 0,125,023 B1; Boss et al., U.S. Patent No. 4,816,397; Boss et al., European Patent No. 0,120,694 B1; Neuberger, MS et al., WO 86/01533 ; Neuberger, MS, et al., European Patent No. 0, 194, 276 B1; Winter , U.S. Patent No. 5 , 225, 539; Winter , European Patent No. 0, 239, 400 B1; Padlan, EA, et al., European Patent Application No. 0,519,596 A1. For a single-chain antibody, see also: Ladner et al., U.S. Patent No. 4,946,778; Huston , U.S. Patent No. 5,476,786; and Bird, RE et al., Science , 242: 423-426 (1988). In some embodiments, the human immunoglobulin is a deimmunized antibody. See, for example, Carr et al., U.S. Patent No. 7,264,806, which is directed to a de-immunized immunoglobulin that has been modified to reduce the number of potential T-cell epitopes, thereby reducing the propensity of immunoglobulins to elicit an immune response when administered to humans. .

在特別具體實施例,人類化免疫球蛋白包含一或更多下列小鼠單株抗體的一或更多輕鏈CDR及一或更多重鏈CDR:小鼠8G3.25.3.5、小鼠4G7.F3、小鼠9D9.A2、小鼠11C11.C5、小鼠3G7.E9、小鼠5F7.1.1.4、小鼠12G6.15.1.2、小鼠23E6.2.2.1、小鼠2C3.3.8.1、小鼠7F11.1.9.7、及小鼠4B10.1.2.4。In a particular embodiment, the humanized immunoglobulin comprises one or more of the following light chain CDRs of the mouse monoclonal antibody and one or more heavy chain CDRs: mouse 8G3.25.3.5, mouse 4G7 .F3, mouse 9D9.A2, mouse 11C11.C5, mouse 3G7.E9, mouse 5F7.1.1.4, mouse 12G6.15.1.2, mouse 23E6.2.2.1, mouse 2C3.3.8 .1, mouse 7F11.1.9.7, and mouse 4B10.1.2.4.

在另一具體實施例,人類化免疫球蛋白結合人類CD52的親合性類似於或較佳於Campath。在特別具體實施例,本發明人類化免疫球蛋白具本發明小鼠抗-人類CD52抗體的結合專一性(例如,具人類CD52的專一性,具相同或類似抗原決定區專一性)及/或其具相同抑制功能。人類化免疫球蛋白可具此處所敘述小鼠抗-人類CD52抗體或人類化抗-人類CD52抗體的結合專一性及/或抑制活性,及/或此處所敘述小鼠抗-人類CD52抗體或人類化抗-人類CD52抗體的抗原決定區專一性(例如,其可與小鼠抗-人類CD52抗體競爭,或是另一種人類化抗-CD52抗體(例如,Campath)以結合至CD52,及/或其可具小鼠或人類化抗-人類CD52抗體的抑制功能)。在特別具體實施例,人類化免疫球蛋白具小鼠抗體8G3、4G7、9D9、11C11、3G7、5F7、12G6、23E6、2C3、7F11、及r4B10中任一個的結合專一性、抗原決定區專一性及/或抑制活性。In another embodiment, the affinity of the humanized immunoglobulin to bind to human CD52 is similar or preferred to Campath . In a particular embodiment, the humanized immunoglobulin of the invention has the binding specificity of a mouse anti-human CD52 antibody of the invention ( eg , specificity of human CD52, with the same or similar epitope specificity) and/or It has the same suppression function. A humanized immunoglobulin can have the binding specificity and/or inhibitory activity of a mouse anti-human CD52 antibody or a humanized anti-human CD52 antibody as described herein, and/or a mouse anti-human CD52 antibody or human described herein. The specificity of the epitope of a human anti-human CD52 antibody ( eg , it can compete with a mouse anti-human CD52 antibody, or another humanized anti-CD52 antibody ( eg, Campath) ) to bind to CD52, and/or it may have the inhibitory function of a mouse or humanized anti-human CD52 antibody). In a specific embodiment, the humanized immunoglobulin has binding specificity, antigenic determining region specificity of any of mouse antibodies 8G3, 4G7, 9D9, 11C11, 3G7, 5F7, 12G6, 23E6, 2C3, 7F11, and r4B10. And/or inhibit activity.

作為人類來源的人類化免疫球蛋白部份或是免疫球蛋白鏈(例如,骨架區;恆定區)的部份可得自任何合適的人類化免疫球蛋白或是免疫球蛋白鏈。例如,在人類化或嵌合抗體中的人類恆定區或其部份可得自人類κ或λ輕鏈基因,及/或得自人類γ(例如,γ1、γ2、γ3、γ4)、μ、α(例如,α1、α2)、d或e重鏈基因,其包含對偶基因變異體。一特定的恆定區(例如,IgG1),其變異體或部分可被選擇以適合效應遺傳因子功能。例如,經突變恆定區(變異體)可被併入免疫球蛋白或是免疫球蛋白鏈以最小化至Fc受體的結合及/或固定補體的能力,(參看例如,Winter等,GB 2,209,757 B;Morrison.,WO 89/07142;Morgan等WO 94/29351,December 22,1994)。在一具體實施例中,人類骨架區於其結構或序列中沒有任何變異或突變。在特別具體實施例中,骨架區為一種於其序列中不具任何突變或變異的生殖株骨架序列。A portion of a humanized immunoglobulin as a human source or a portion of an immunoglobulin chain ( eg, a framework region; a constant region) can be obtained from any suitable humanized immunoglobulin or immunoglobulin chain. For example, a human constant region or portion thereof in a humanized or chimeric antibody can be derived from a human kappa or lambda light chain gene, and/or from human gamma (eg, gamma 1, gamma 2, gamma 3, gamma 4), μ, An alpha ( eg, alpha 1, alpha 2), d or e heavy chain gene comprising a dual gene variant. A particular constant region ( eg, IgGl), a variant or portion thereof, can be selected to suit the effector gene function. For example, a mutant constant region (variant) can be incorporated into an immunoglobulin or immunoglobulin chain to minimize the ability to bind to the Fc receptor and/or to fix complement (see, eg, Winter et al, GB 2,209,757 B). ; Morrison et al ., WO 89/07142; Morgan et al. WO 94/29351, December 22, 1994). In a specific embodiment, the human framework region does not have any variation or mutation in its structure or sequence. In a particular embodiment, the framework region is a germline backbone sequence that does not have any mutations or variations in its sequence.

當用於此處時,名稱「生殖株」係表示抗體基因及基因區段的核苷酸序列及胺基酸序列,因為它們經由生殖細胞自母代傳代至子代。此生殖株序列與編碼成熟B細胞中抗體的核苷酸序列不同,成熟B細胞在B細胞成熟進行期間已由重組及超突變事件變更。「利用」特定生殖株的抗體具與生殖株核苷酸序列或是與其指定胺基酸序列最接近的核苷酸或胺基酸序列,與生殖株序列相較此種抗體常為突變的。When used herein, the designation "reproductive strain" refers to the nucleotide sequence of the antibody gene and gene segment and the amino acid sequence as they are passaged from the mother to the progeny via the germ cells. This genital sequence differs from the nucleotide sequence encoding the antibody in mature B cells, which have been altered by recombination and hypermutation events during B cell maturation. The antibody that "utilizes" a particular reproductive strain has a nucleotide sequence closest to its reproductive strain or a nucleotide or amino acid sequence closest to its assigned amino acid sequence, and such antibodies are often mutated compared to the sequence of the reproductive strain.

在其他具體實施例中,人類骨架於其結構或序列中具來自生殖株序列的最少變異或突變(例如,少於3、4、5、6、7、8、9或10個受體骨架殘基已使用授予體骨架殘基取代以改善結合親合力,參看Queen,美國專利第5,530,101號)。在特別具體實施例中,人類化免疫球蛋白鏈的骨架中有限數目的胺基酸(例如,1、2、3、4、5、6、7、8、9或10個胺基酸)係選擇為與在授予體序列這些位置的胺基酸相同(亦即,"回復突變"),而非與受體序列相同,以增加包含用於人類CD52的人類化免疫球蛋白鏈的抗體之親合力。In other embodiments, the human framework has minimal variation or mutations in the structure or sequence from the sequence of the reproductive line (eg, less than 3, 4, 5, 6, 7, 8, 9, or 10 receptor backbone residues) The base has been substituted with a donor backbone residue to improve binding affinity, see Queen et al ., U.S. Patent No. 5,530,101). In a particular embodiment, a limited number of amino acids (eg, 1, 2, 3, 4, 5, 6, 7, 8, 9 or 10 amino acids) in the backbone of the humanized immunoglobulin chain are It is selected to be the same as the amino acid at these positions in the donor sequence (ie, "backmutation"), but not the receptor sequence, to increase the affinity of the antibody comprising the humanized immunoglobulin chain for human CD52. Together.

人類骨架區(例如,重及/或輕鏈變異區)較佳為得自或衍生自具序列與授予體免疫球蛋白(小鼠抗-CD52抗體)的抗原-結合區域的類似或相當區域(例如,重及/或輕鏈變異區)相似的人類抗體變異區。人類化免疫球蛋白的人類來源部份的骨架區其他來源包含人類變異區一致性序列(參看例如,Kettleborough,C. A..,Protein Engineering 4:773-783(1991);CarterWO 94/04679;Carter美國專利第6,407,213號))。例如,用於得到非人類部份的抗體授予體序列的區域(例如,變異區序列)可與人類序列相比較,如Kabat,E. A.等Sequences of Proteins of Immunological Interest,Fifth Edition,U.S. Department of Health and Human Services,U.S. Government Printing Office(1991)中所述選擇人類化免疫球蛋白的人類部份的特定來源,例如,骨架區來源。The human framework region (eg, heavy and/or light chain variant regions) is preferably derived or derived from a similar or comparable region of the antigen-binding region of the sequence with the donor immunoglobulin (mouse anti-CD52 antibody) ( For example, heavy and/or light chain variant regions are similar to human antibody variant regions. Other sources of the framework region of the human-derived portion of the human immunoglobulin comprise human variant region consensus sequences (see, for example, Kettleborough, CA et al ., Protein Engineering 4: 773-783 (1991); Carter et al. WO 94/04679; Carter U.S. Patent No. 6,407,213)). For example, a region (eg, a variant region sequence) for obtaining an antibody-granting sequence of a non-human portion can be compared to a human sequence, such as Kabat, EA, etc., Sequences of Proteins of Immunological Interest , Fifth Edition, US Department of Health and A specific source of human parts of humanized immunoglobulins, such as the source of the framework regions, is selected as described in Human Services, US Government Printing Office (1991).

在一具體實施例中,人類化免疫球蛋白鏈的骨架區係得自,或衍生自具與非人類授予體變異區至少約50%,至少約55%,至少約60%,至少約65%,至少約70%,至少約75%,至少約80%,至少約85%,至少約90%或至少約95%的總序列相似性,的人類Ig變異區。在特別具體實施例中,人類化免疫球蛋白鏈的骨架區係得自或衍生自具與非人類授予體免疫球蛋白變異區的骨架區至少約50%,至少約55%,至少約60%,至少約65%,至少約70%,至少約75%,至少約80%,至少約85%,至少約90%,或至少約95%的總序列相似性,的人類變異區骨架區。In a specific embodiment, the framework region of the humanized immunoglobulin chain is derived from, or derived from, at least about 50%, at least about 55%, at least about 60%, at least about 65% of the variant region with the non-human donor. , at least about 70%, at least about 75%, at least about 80%, at least about 85%, at least about 90% or at least about 95% of the total sequence similarity of the human Ig variant region. In a particular embodiment, the framework region of the humanized immunoglobulin chain is derived or derived from at least about 50%, at least about 55%, at least about 60% of the framework region of the immunoglobulin variant region with the non-human donor. At least about 65%, at least about 70%, at least about 75%, at least about 80%, at least about 85%, at least about 90%, or at least about 95% of the total sequence similarity of the human variant region framework region.

在一具體實施例中,人類化免疫球蛋白的至少一個骨架區(FR)係得自或衍生自人類來源抗體的一或多個鏈,於是,FR可包含得自或衍生自人類來源的一或多個抗體(例如,得自人類免疫球蛋白鏈,得自人類一致性序列)的FR1及/或FR2及/或FR3及/或FR4。In a specific embodiment, at least one framework region (FR) of the humanized immunoglobulin is derived or derived from one or more strands of a human-derived antibody, such that the FR can comprise one derived or derived from a human source. Or FR1 and/or FR2 and/or FR3 and/or FR4 of multiple antibodies (eg, derived from human immunoglobulin chains, derived from human consensus sequences).

用於本發明的免疫球蛋白部份具相同,或類似於它們所衍生自的免疫球蛋白或是其變異物的序列。此種變異物包含因加成、消除或取代(例如,保守型取代)一或多個殘基而不同的突變物,例如,藉由一或多個加成、消除或取代而與母續列相差多至3、4、5、6、7、8、9或10個殘基。如上文所指出,本發明的人類化免疫球蛋白包含來自此處所敘述一或多個小鼠抗-CD52抗體(授予體抗體)的一或多個CDR。在骨架區的變化可被進行,例如以來自授予體抗體相對應位置的殘基取代人類來源骨架區的殘基。一或多個突變可被進行,其包含在骨架區的一或多個胺基酸的消除、插入及取代。若需要,可包含骨架突變於人類化抗體或鏈,及突變部位可使用任何合適方法,例如如在WO 98/06248所敘述選擇之,其整個意旨係併入做為參考。The immunoglobulin moieties used in the present invention are identical or similar in sequence to the immunoglobulin from which they are derived or variants thereof. Such variants include mutants that differ by addition, elimination or substitution (eg, conservative substitution) of one or more residues, eg, by one or more additions, eliminations or substitutions The difference is up to 3, 4, 5, 6, 7, 8, 9 or 10 residues. As indicated above, the humanized immunoglobulins of the invention comprise one or more CDRs from one or more mouse anti-CD52 antibodies (granting antibodies) as described herein. Variations in the framework regions can be performed, for example, by replacing residues from the human-derived framework regions with residues from the corresponding positions of the donor antibody. One or more mutations can be made which comprise elimination, insertion and substitution of one or more amino acids in the framework region. If desired, a backbone mutation can be included in the humanized antibody or strand, and the site of the mutation can be any suitable method, for example, as described in WO 98/06248, the entire disclosure of which is incorporated herein by reference.

熟知該技藝者了解在一些情況與小鼠抗-CD52抗體的一或更多CDRs側面相接的殘基會貢獻,及在一些情況,為直接或間接地為功能(例如,結合)所需要。如此,在一些具體實施例中,與小鼠骨架的一或多個CDR側面相接的一或多個胺基酸(例如,1、2、3、4、5、6、7、8、9、10個側接胺基酸)亦包含於人類化免疫球蛋白。It is well known to those skilled in the art that in some cases residues that are flanked by one or more CDRs of a mouse anti-CD52 antibody will contribute, and in some cases, are required for direct or indirect function (e.g., binding). Thus, in some embodiments, one or more amino acids that are flanked by one or more CDR sides of the mouse backbone (eg, 1, 2, 3, 4, 5, 6, 7, 8, 9 , 10 side-linked amino acids are also included in humanized immunoglobulins.

在一些具體實施例中,本發明的人類化抗體的重鏈骨架區利用人類VH3-72或VH3-23生殖株序列。在一些具體實施例中,本發明的人類化抗體的人類輕鏈骨架區利用人類Vk2-A18b生殖株序列。回復突變可如在下文工作實例所敘述選擇性地於一或多個殘基在這些FR區域進行以改善人類化抗體的CD52-結合親合力。In some embodiments, the heavy chain framework regions of the humanized antibodies of the invention utilize human VH3-72 or VH3-23 reproductive strain sequences. In some embodiments, the human light chain backbone region of the humanized antibody of the invention utilizes the human Vk2-A18b genital sequence. Back mutations can be performed selectively in one or more residues in these FR regions as described in the working examples below to improve the CD52-binding affinity of the humanized antibody.

「親合力」為一種技藝名稱,其敘述結合交互作用的強度及典型上係指免疫球蛋白對人類CD52的結合整體強度。"Affinity" is a technical name that describes the strength of the binding interaction and typically refers to the overall strength of the immunoglobulin binding to human CD52.

在特別具體實施例,免疫球蛋白具EC50值小於10微克/毫升(例如,由流式細胞計數法計數所決定)的結合活性。在另一具體實施例,免疫球蛋白具EC50值小於5.0微克/毫升,或小於1.0微克/毫升(例如,由流式細胞計數所決定)的結合活性。In particular, binding activity specific embodiments, the immunoglobulin with EC 50 values of less than 10 [mu] g / ml (e.g., determined by flow cytometry counts). In another embodiment, the immunoglobulin with EC 50 values of less than 5.0 g / ml, or less than 1.0 g / ml (e.g., determined by flow cytometry) binding activity.

在一些具體實施例,免疫球蛋白以300奈莫耳濃度至1微微莫耳濃度(亦即,3 x 10-7至1 x 10-12莫耳濃度),較佳為50奈莫耳濃度至1微微莫耳濃度,更佳為5奈莫耳濃度至1微微莫耳濃度及最佳為1奈莫耳濃度至1微微莫耳濃度的親合力(KD;KD=Koff(kd)/Kon(ka))結合至人類CD52,例如,由表面電漿共振所決定的,1 x 10-7莫耳濃度或更少,較佳為1 x 10-8莫耳濃度或更少,更佳為1 x 10-9莫耳濃度或更少,有利的是1 x 10-10莫耳濃度或更少及最佳為1 x 10-11莫耳濃度或1 x 10-12莫耳濃度或更少的KD;及/或5 x 10-1秒-1至1 x 10-7秒-1,較佳為1 x 10-2秒-1至1 x 10-6秒-1,更佳為5 x 10-3秒-1至1 x 10-5秒-1的Koff速率常數,,例如5 x 10-1秒-1或更少,較佳為1 x 10-2秒-1或更少,有利的是1 x 10-3秒-1或更少,更佳為1 x 10-4秒-1或更少,更佳為1 x 10-5秒-1或更少,及最佳為1 x 10-6秒-1或更少。In some embodiments, the immunoglobulin is at a concentration of 300 nanomolar to a concentration of 1 picomol (ie, 3 x 10 -7 to 1 x 10 -12 molar), preferably 50 nanomolar to 1 picomolar concentration, more preferably 5 nanomolar to 1 micromolar and most preferably 1 nanomolar to 1 picomolar concentration (K D ; K D = K off (kd) /Kon(ka)) binds to human CD52, for example, determined by surface plasma resonance, 1 x 10 -7 molar concentration or less, preferably 1 x 10 -8 molar concentration or less, more Good for 1 x 10 -9 moles or less, advantageously 1 x 10 -10 moles or less and optimally 1 x 10 -11 moles or 1 x 10 -12 moles or Less K D ; and / or 5 x 10 -1 sec -1 to 1 x 10 -7 sec -1, preferably 1 x 10 -2 sec -1 to 1 x 10 -6 sec -1, more preferably a K off rate constant of 5 x 10 -3 sec -1 to 1 x 10 -5 sec -1, for example 5 x 10 -1 sec -1 or less, preferably 1 x 10 -2 sec -1 or Less, advantageously 1 x 10 -3 sec -1 or less, more preferably 1 x 10 -4 sec -1 or less, more preferably 1 x 10 -5 sec -1 or less, and most Good for 1 x 10 -6 seconds -1 or less.

熟知該技藝者可了解,可使用各種方法以確認根據此處所提供及在該技藝所已知方法所製造的免疫球蛋白具必要專一性(例如,結合專一性,抗原決定區專一性)。例如,具用於人類CD52的結合專一性的本發明之人類化抗-CD52免疫球蛋白之結合功能可使用任何合適方法偵測,例如,監控人類化免疫球蛋白與人類CD52之間複合物的形成(例如,包含人類CD52的膜部分;攜帶人類CD52的細胞,例如人類T細胞、人類B細胞;CHO細胞或包含及表現編碼人類CD52的核酸之重組宿主細胞;具CD52胺基酸序列的肽(例如,合成肽);包含人類CD52的實體支撐)之試驗。It will be appreciated by those skilled in the art that various methods can be used to confirm the necessary specificity (e.g., specificity, epitope-specificity) of immunoglobulins made according to methods provided herein and known in the art. For example, the binding function of the humanized anti-CD52 immunoglobulin of the present invention having binding specificity for human CD52 can be detected using any suitable method, for example, monitoring the complex between humanized immunoglobulin and human CD52. Forming (eg, a membrane portion comprising human CD52; a cell carrying human CD52, such as a human T cell, a human B cell; a CHO cell or a recombinant host cell comprising and expressing a nucleic acid encoding human CD52; a peptide having a CD52 amino acid sequence (eg, synthetic peptides; experiments involving the physical support of human CD52).

本發明的免疫球蛋白(例如,本發明人類化免疫球蛋白)結合至人類CD52上相同抗原決定區做為特別小鼠,嵌合,或人類化單株抗體,或是結合至與特別小鼠,嵌合,或人類化單株抗體所結合的人類CD52上抗原決定區重疊的人類CD52上抗原決定區的能力,可使用熟知該技藝者已知各種技術(包含例如競爭性結合試驗)容易地決定。這些技術涉及使用該特別抗體的標記形式,及在本發明免疫球蛋白存在及不存在情況下經標記抗體至人類CD52的結合之量度。The immunoglobulin of the present invention (for example, the humanized immunoglobulin of the present invention) binds to the same epitope in human CD52 as a special mouse, chimeric, or humanized monoclonal antibody, or binds to a specific mouse. The ability of the chimeric, or humanized monoclonal antibody to bind to the epitope on human CD52 overlying the epitope of human CD52, can be readily accomplished using various techniques known to those skilled in the art, including, for example, competitive binding assays. Decide. These techniques involve the use of a labeled form of the particular antibody, and a measure of the binding of the labeled antibody to human CD52 in the presence and absence of an immunoglobulin of the invention.

「抗原決定區」當用於此處時係包含能夠特定結合至免疫球蛋白的任何蛋白決定基。抗原決定區決定基一般由分子例如胺基酸或碳水化合物或糖側鏈的化學活性表面分組組成及一般具特定三度空間結構特徵,與特定電荷特徵。抗原決定區可為「線型的」或「構形的」。在線型抗原決定區,在蛋白及交互作用分子(例如抗體)之間的所有交互作用點沿蛋白的一級胺基酸序列線形發生。在構形抗原決定區,交互作用點跨越在彼此分開的蛋白上的胺基酸殘基發生。一旦決定抗原上的所欲抗原決定區,可例如使用於本發明所敘述技術產生抗體至該抗原決定區。或者,在發現方法期間,抗體的產生及特徵化可說明關於所欲抗原決定區的資料,由此資料,可接著競爭性地篩選抗體以結合至相同抗原決定區。達到此目的的一個方法為進行競爭性研究以發現彼此競爭性結合的抗體,亦即,為結合至抗原競爭的抗體。An "antigenic region", when used herein, includes any protein determinant capable of specifically binding to an immunoglobulin. The epitope-determining group is typically composed of chemically active surface groups of molecules such as amino acids or carbohydrate or sugar side chains and generally has specific tertiary spatial structural characteristics, with specific charge characteristics. The epitope can be "linear" or "configurable". Inline-type epitopes, all interactions between proteins and interacting molecules (eg, antibodies) occur linearly along the primary amino acid sequence of the protein. In the conformational epitope, the interaction point occurs across amino acid residues on proteins that are separated from each other. Once the desired epitope on the antigen is determined, the antibody can be produced to the epitope, for example, using the techniques described herein. Alternatively, during discovery of the method, the production and characterization of the antibody can be indicative of information about the desired epitope, whereby the data can then be competitively screened for binding to the same epitope. One way to achieve this is to conduct competitive studies to find antibodies that compete for binding to each other, that is, antibodies that compete for binding to the antigen.

在一個實施例中,為決定測試抗體是否結合至本發明人類化抗體的相同或重疊抗原決定區,我們使得本發明抗-CD52抗體在飽和條件下結合至CD52及接著量度測試抗體結合至CD52的能力。若測試抗體能夠如參考抗-CD52抗體在同時間結合至CD52,則測試抗體結合至與參考抗-CD52抗體不同的抗原決定區,然而,若測試抗體不能在同時間結合至CD52,則測試抗體結合至相同抗原決定區,重疊抗原決定區,或是緊鄰由本發明抗-CD52抗體所結合之抗原決定區的抗原決定區。此實驗可使用ELISA、RIA、BIACORETM、或流式細胞計數執行。為測試抗-CD52抗體是否與其他抗-CD52抗體交叉競爭,我們可在兩個方向使用上文所敘述競爭方法,亦即,決定參考抗體是否阻擋測試抗體及反之亦然。在一較佳具體實施例中,實驗係使用BIACORETM執行。In one embodiment, to determine whether a test antibody binds to the same or overlapping epitopes of a humanized antibody of the invention, we allow the anti-CD52 antibody of the invention to bind to CD52 under saturating conditions and subsequently measure the binding of the antibody to CD52. ability. If the test antibody is capable of binding to CD52 at the same time as the reference anti-CD52 antibody, the test antibody binds to a different epitope than the reference anti-CD52 antibody, however, if the test antibody cannot bind to CD52 at the same time, the test antibody Binding to the same epitope, overlapping epitopes, or epitopes adjacent to the epitope determined by the anti-CD52 antibody of the invention. This experiment can be used ELISA, RIA, BIACORE TM, or flow cytometry performed. To test whether an anti-CD52 antibody cross-competes with other anti-CD52 antibodies, we can use the competition method described above in both directions, ie, to determine whether the reference antibody blocks the test antibody and vice versa. In a preferred embodiment, the experimental system using BIACORE TM performed.

組合亦有用於特徵化本發明抗體,「組合」這名稱係表示基於其抗原結合特徵以分組抗體的方法。一種基於其交叉競爭以「組合」抗體的高效能方法係描述於國際專利申請案第WO 03/48731號。Combinations are also used to characterize antibodies of the invention, and the term "combination" refers to a method of grouping antibodies based on their antigen binding characteristics. A high performance method based on its cross-competition to "combine" antibodies is described in International Patent Application No. WO 03/48731.

亦於此處提供的是人類化免疫球蛋白的部份,例如輕鏈、重鏈及輕及重鏈的部份。這些免疫球蛋白部份可得自或衍生自免疫球蛋白(例如,藉由還原及/或裂解),或是由具所欲性質(例如,鍵結人類CD52,序列類似性)的核酸編碼一部份免疫球蛋白或其鏈來製造或表現,它們可由例如相關部份的重新合成所製備。包含人類及非人類來源所欲部份(例如,抗原結合區域、CDR、FR、C區域)的人類化免疫球蛋白可使用合成及/或重組核酸製造以製備編碼所欲人類化鏈的構成物(例如,cDNA),例如,為製備一部份免疫球蛋白(例如,一部份鏈),可於所欲位置引入一或多個中止密碼子。為人類化變異區編碼的核酸(例如,DNA)序列可使用PCR突變誘發方法建構以變更現有DNA序列(參看例如,Kamman,M.,等,Nucl. Acids Res. 17:5404(1989))。為新CDRs編碼的PCR引子可雜交為先前人類化變異區的DNA模版,其係基於相同,或非常類似的,人類變異區(Sato,K.,等,Cancer Research 53:851-856(1993))。若無法以類似DNA序列用做模版,包含編碼變異區序列的序列之核酸可由合成性寡核甘酸構建(參看例如,Kolbinger,F.,Protein Engineering 8:971-980(1993))。編碼信號胜肽的序列亦可併入核酸(例如,於合成時,於插入載體時),若沒有信號胜肽序列(例如,典型上不存在),可使用來自其他抗體的信號胜肽序列(參看例如,Kettleborough,C.A.,Protein Engineering 4:773-783(1991))。使用這些方法,此處所敘述方法或其他合適方法,變異物可容易的被製造。Also provided herein are portions of human immunoglobulins, such as light chains, heavy chains, and light and heavy chain portions. These immunoglobulin moieties may be derived or derived from immunoglobulins ( eg, by reduction and/or cleavage) or may be encoded by a nucleic acid having the desired properties (eg, binding human CD52, sequence similarity). Part of the immunoglobulin or its chains are made or expressed, and they can be prepared, for example, by resynthesis of related moieties. Humanized immunoglobulins comprising portions of human and non-human origin (eg, antigen binding regions, CDRs, FRs, C regions) can be made using synthetic and/or recombinant nucleic acids to prepare constructs encoding the desired humanized strand. ( e.g., cDNA), for example, to prepare a portion of an immunoglobulin ( e.g., a portion of a strand), one or more stop codons can be introduced at the desired position. Nucleic acid ( e.g., DNA) sequences encoding humanized variant regions can be constructed using PCR mutation inducing methods to alter existing DNA sequences (see, e.g., Kamman, M., et al, Nucl. Acids Res. 17: 5404 (1989)). PCR primers encoding new CDRs can hybridize to DNA templates of previously humanized variant regions based on the same, or very similar, human variant regions (Sato, K., et al, Cancer Research 53: 851-856 (1993) ). If a template is not used as a DNA sequence, the nucleic acid comprising the sequence encoding the sequence of the variant region can be constructed from a synthetic oligonucleotide (see, for example, Kolbinger, F., Protein Engineering 8: 971-980 (1993)). The sequence encoding the signal peptide can also be incorporated into a nucleic acid ( eg, upon insertion into a vector), and if no signal peptide sequence is present ( eg, typically absent), a signal peptide sequence from other antibodies can be used ( See, for example, Kettleborough, CA, Protein Engineering 4:773-783 (1991)). Variants can be readily fabricated using these methods, methods described herein, or other suitable methods.

本發明係關於一種人類化免疫球蛋白,其具對人類CD52的結合專一性及包含人類化輕鏈及人類化重鏈及/或其部份。在一個實施例中,人類化免疫球蛋白包含一種含有SEQ ID NO:3的一或多個CDR(例如,所有三個CDR)的輕鏈及一種含有SEQ ID NO:16的一或多個CDR(例如,所有三個CDR)的重鏈;一種含有SEQ ID NO:4的一或多個CDR(例如,所有三個CDR)的輕鏈及一種含有SEQ ID NO:17的一或多個CDR(例如,所有三個CDR)的重鏈;一種含有SEQ ID NO:5的一或多個CDR(例如,所有三個CDR)的輕鏈及一種含有SEQ ID NO:18的一或多個CDR(例如,所有三個CDR)的重鏈;一種含有SEQ ID NO:6的一或多個CDR(例如,所有三個CDR)的輕鏈及一種含有SEQ ID NO:19的一或多個CDR的重鏈;一種含有SEQ ID NO:7的一或多個CDR(例如,所有三個CDR)的輕鏈及一種含有SEQ ID NO:20的一或多個CDR(例如,所有三個CDR)的重鏈;一種含有SEQ ID NO:8的一或多個CDR(例如,所有三個CDR)的輕鏈及一種含有SEQ ID NO:21的一或多個CDR(例如,所有三個CDR)的重鏈;一種含有SEQ ID NO:9的一或多個CDR(例如,所有三個CDR)的輕鏈及一種含有SEQ ID NO:22的一或多個CDR(例如,所有三個CDR)的重鏈;一種含有SEQ ID NO:10的一或多個CDR(例如,所有三個CDR)的輕鏈及一種含有SEQ ID NO:23的一或多個CDR(例如,所有三個CDR)的重鏈;一種含有SEQ ID NO:11的一或更多CDR(例如,所有三個CDR)的輕鏈及一種含有SEQ ID NO:24的一或多個CDR(例如,所有三個CDR)的重鏈;一種含有SEQ ID NO:12的一或多個CDR(例如,所有三個CDR)的輕鏈及一種含有SEQ ID NO:25的一或多個CDR(例如,所有三個CDR)的重鏈;一種含有SEQ ID NO:13的一或多個CDR(例如,所有三個CDR)的輕鏈及一種含有SEQ ID NO:26的一或多個CDR(例如,所有三個CDR)的重鏈。The present invention relates to a humanized immunoglobulin having binding specificity for human CD52 and comprising a humanized light chain and a humanized heavy chain and/or a portion thereof. In one embodiment, the humanized immunoglobulin comprises a light chain comprising one or more CDRs of SEQ ID NO: 3 ( eg, all three CDRs) and one or more CDRs comprising SEQ ID NO: (e.g., all three CDR) of a heavy chain; containing SEQ ID NO: 4, a CDR or more (e.g., all three CDR) and a light chain containing SEQ ID NO: one or more CDR. 17 (e.g., all three CDR) of a heavy chain; containing SEQ ID NO:. 5 one or more CDR (e.g., all three CDR) and a light chain containing SEQ ID NO: 18 one or more of the CDR (e.g., all three CDR) of a heavy chain; containing SEQ ID NO: 6, a CDR or more (e.g., all three CDR) and a light chain containing SEQ ID NO: 19 one or more of the CDR Heavy chain; a light chain comprising one or more CDRs of SEQ ID NO: 7 ( eg, all three CDRs) and one or more CDRs comprising SEQ ID NO: 20 ( eg, all three CDRs) Heavy chain; a light chain comprising one or more CDRs of SEQ ID NO: 8 ( eg, all three CDRs) and one or more CDRs comprising SEQ ID NO: 21 ( eg, all three CDRs) Heavy chain; one containing SEQ ID NO: 9, one or more CDRs of (e.g., all three CDR) and a light chain containing SEQ ID NO: 22 one or more of the CDRs of (e.g., all three CDR) of a heavy chain; SEQ ID containing NO: 10 or more of the CDRs of a (e.g., all three CDR) and a light chain containing SEQ ID NO: 23 is CDRs of one or more (e.g., all three CDR) of a heavy chain; SEQ ID containing NO: a light chain of one or more CDRs (eg, all three CDRs) of 11 and a heavy chain comprising one or more CDRs of SEQ ID NO: 24 (eg, all three CDRs); one containing SEQ ID NO: 12 one or more of the CDRs of (e.g., all three CDR) and a light chain containing SEQ ID NO: 25 CDRs of one or more (e.g., all three CDR) of a heavy chain; SEQ ID containing NO: a light chain of one or more CDRs (eg, all three CDRs) of 13 and a heavy chain comprising one or more CDRs of SEQ ID NO: 26 (eg, all three CDRs).

在一個實施例中,本發明人類化免疫球蛋白包含重鏈(H)-CDR1、H-CDR2、H-CDR3,輕鏈(L)-CDR1、L-CDR2、及L-CDR3其胺基酸序列為:a)分別是SEQ ID NOs: 51、59、69、29、36及43;b)分別是SEQ ID NOs: 50、60、69、29、37及43;c)分別是SEQ ID NOs: 50、61、68、29、38及43;d)分別是SEQ ID NOs: 50、61、69、29、36及43;e)分別是SEQ ID NOs: 50、62、69、29、39及43;f)分別是SEQ ID NOs: 52、61、70、30、40及43;g)分別是SEQ ID NOs: 53、63、71、31、36及44;h)分別是SEQ ID NOs: 54、64、71、31、36及45;i)分別是SEQ ID NOs: 55、63、72、31、36及46;j)分別是SEQ ID NOs: 56、65、73、32、41及47;k)分別是SEQ ID NOs: 56、65、294、32、41及47,或1)分別是SEQ ID NOs: 56、66、74、33、41及48。In one embodiment, the humanized immunoglobulin of the invention comprises a heavy chain (H)-CDR1, an H-CDR2, an H-CDR3, a light chain (L)-CDR1, an L-CDR2, and an L-CDR3 amino acid thereof. The sequences are: a) SEQ ID NOs: 51, 59, 69, 29, 36 and 43; b) SEQ ID NOs: 50, 60, 69, 29, 37 and 43, respectively; c) SEQ ID NOs, respectively 50, 61, 68, 29, 38 and 43; d) SEQ ID NOs: 50, 61, 69, 29, 36 and 43; e) SEQ ID NOs: 50, 62, 69, 29, 39, respectively And 43; f) are SEQ ID NOs: 52, 61, 70, 30, 40 and 43; g) are SEQ ID NOs: 53, 63, 71, 31, 36 and 44, respectively; h) are SEQ ID NOs, respectively 54, 64, 71, 31, 36 and 45; i) SEQ ID NOs: 55, 63, 72, 31, 36 and 46; j) SEQ ID NOs: 56, 65, 73, 32, 41, respectively And 47; k) are SEQ ID NOs: 56, 65, 294, 32, 41 and 47, respectively, or 1) are SEQ ID NOs: 56, 66, 74, 33, 41 and 48, respectively.

在另一實施例中,本發明人類化免疫球蛋白包含H-CDR3及L-CDR3其序列為a)分別是SEQ ID NOs: 69及43;b) 分別是SEQ ID NOs: 68及43;c)分別是SEQ ID NOs: 70及43;d)分別是SEQ ID NOs: 71及44;e)分別是SEQ ID NOs: 71及45;f)分別是SEQ ID NOs: 72及46;g)分別是SEQ ID NOs: 73及47;h)分別是SEQ ID NOs: 294及47;或i)分別是SEQ ID NOs: 74及48。In another embodiment, the humanized immunoglobulin of the invention comprises H-CDR3 and L-CDR3, the sequence of which is a) SEQ ID NOs: 69 and 43, respectively; b) SEQ ID NOs: 68 and 43; ) SEQ ID NOs: 70 and 43, respectively; d) SEQ ID NOs: 71 and 44; e) SEQ ID NOs: 71 and 45, respectively; f) SEQ ID NOs: 72 and 46; g) respectively Is SEQ ID NOs: 73 and 47; h) are SEQ ID NOs: 294 and 47, respectively; or i) are SEQ ID NOs: 74 and 48, respectively.

在具體實施例中,人類化免疫球蛋白具對人類CD52的結合專一性及包含一種輕鏈,其包含由SEQ ID NO:27、SEQ ID NO:28、SEQ ID NO:29、SEQ ID NO:30、SEQ ID NO:31、SEQ ID NO:32、SEQ ID NO:33、SEQ ID NO:34、SEQ ID NO:35、SEQ ID NO:36、SEQ ID NO:37、SEQ ID NO:38、SEQ ID NO:39、SEQ ID NO:40、SEQ ID NO:41、SEQ ID NO:42、SEQ ID NO:43、SEQ ID NO:44、SEQ ID NO:45、SEQ ID NO:46、SEQ ID NO:47及SEQ ID NO:48所組成族群選出的一或多個CDR,或是其組合;及一種重鏈,其包含由SEQ ID NO:49、SEQ ID NO:50、SEQ ID NO:51、SEQ ID NO:52、SEQ ID NO:53、SEQ ID NO:54、SEQ ID NO:55、SEQ ID NO:56、SEQ ID NO:57、SEQ ID NO:58、SEQ ID NO:59、SEQ ID NO:60、SEQ ID NO:61、SEQ ID NO:62、SEQ ID NO:63、SEQ ID NO:64、SEQ ID NO:65、SEQ ID NO:66、SEQ ID NO:67、SEQ ID NO:68、SEQ ID NO:69、SEQ ID NO:70、SEQ ID NO:71、SEQ ID NO:72、SEQ ID NO:73、SEQ ID NO:74及SEQ ID NO:294所組成族群選出的一或多個CDR,或是其組合,其中該人類化免疫球蛋白不為CampathIn a specific embodiment, the humanized immunoglobulin has binding specificity for human CD52 and comprises a light chain comprising SEQ ID NO:27, SEQ ID NO:28, SEQ ID NO:29, SEQ ID NO: 30. SEQ ID NO: 31, SEQ ID NO: 32, SEQ ID NO: 33, SEQ ID NO: 34, SEQ ID NO: 35, SEQ ID NO: 36, SEQ ID NO: 37, SEQ ID NO: 38, SEQ ID NO: 39, SEQ ID NO: 40, SEQ ID NO: 41, SEQ ID NO: 42, SEQ ID NO: 43, SEQ ID NO: 44, SEQ ID NO: 45, SEQ ID NO: 46, SEQ ID NO: 47 and one or more CDRs selected from the group consisting of SEQ ID NO: 48, or a combination thereof; and a heavy chain comprising SEQ ID NO: 49, SEQ ID NO: 50, SEQ ID NO: 51 SEQ ID NO: 52, SEQ ID NO: 53, SEQ ID NO: 54, SEQ ID NO: 55, SEQ ID NO: 56, SEQ ID NO: 57, SEQ ID NO: 58, SEQ ID NO: 59, SEQ ID NO: 60, SEQ ID NO: 61, SEQ ID NO: 62, SEQ ID NO: 63, SEQ ID NO: 64, SEQ ID NO: 65, SEQ ID NO: 66, SEQ ID NO: 67, SEQ ID NO :68, one selected from the group consisting of SEQ ID NO: 69, SEQ ID NO: 70, SEQ ID NO: 71, SEQ ID NO: 72, SEQ ID NO: 73, SEQ ID NO: 74, and SEQ ID NO: 294 Or multiple CDRs, or a combination thereof, In the human immunoglobulin is not Campath .

在另一實施例中,具對人類CD52結合專一性的人類化免疫球蛋白包含一種輕鏈,其包含SEQ ID NO:3、SEQ ID NO:4、SEQ ID NO:5、SEQ ID NO:6、SEQ ID NO:7、SEQ ID NO:8、SEQ ID NO:9、SEQ ID NO:10、SEQ IDNO:11、SEQ ID NO:12或SEQ ID NO:13的一或多個CDR(例如,所有三個CDR),及一種重鏈,其包含SEQ ID NO:16、SEQ ID NO:17、SEQ ID NO:18、SEQ ID NO:19、SEQ ID NO:20、SEQ ID NO:21、SEQ ID NO:22、SEQ ID NO:23、SEQ ID NO:24、SEQ ID NO:25、SEQ ID NO:26或SEQ ID NO: 137的一或多個CDR(例如,所有三個CDR),其中該人類化免疫球蛋白不為CampathIn another embodiment, the humanized immunoglobulin having specificity for human CD52 binding comprises a light chain comprising SEQ ID NO:3, SEQ ID NO:4, SEQ ID NO:5, SEQ ID NO:6 One or more CDRs of SEQ ID NO: 7, SEQ ID NO: 8, SEQ ID NO: 9, SEQ ID NO: 10, SEQ ID NO: 11, SEQ ID NO: 12 or SEQ ID NO: 13 (eg, All three CDRs), and a heavy chain comprising SEQ ID NO: 16, SEQ ID NO: 17, SEQ ID NO: 18, SEQ ID NO: 19, SEQ ID NO: 20, SEQ ID NO: 21, SEQ ID NO: 22, SEQ ID NO: 23, SEQ ID NO: 24, SEQ ID NO: 25, SEQ ID NO: 26 or SEQ ID NO: 137 one or more CDRs (eg, all three CDRs), wherein The human immunoglobulin is not for Campath .

本發明亦相關於一種此處所敘述人類化免疫球蛋白的人類化免疫球蛋白輕鏈。在一個實施例中,該人類化免疫球蛋白輕鏈包含SEQ ID NO:27、SEQ ID NO:28、SEQ ID NO:29、SEQ ID NO:30、SEQ ID NO:31、SEQ ID NO:32、SEQ ID NO:33、SEQ ID NO:34、SEQ ID NO:35、SEQ ID NO:36、SEQ ID NO:37、SEQ ID NO:38、SEQ ID NO:39、SEQ ID NO:40、SEQ ID NO:41、SEQ ID NO:42、SEQ ID NO:43、SEQ ID NO:44、SEQ ID NO:45、SEQ ID NO:46、SEQ ID NO:47、及SEQ ID NO:48所組成族群選出的一或多個CDR,及其組合,其中該人類化免疫球蛋白輕鏈不為Campath的輕鏈。例如,該人類化抗體具L-CDR1、L-CDR2及L-CDR3其胺基酸序列:a)分別為SEQ ID NOs: 29、36及43;b)分別為SEQ ID NOs: 29、37及43;c)分別為SEQ ID NOs: 29、38及43;d)分別為SEQ ID NOs: 29、36及43;e)分別為SEQ ID NOs: 29、39及43;f)分別為SEQ ID NOs: 30、40及43;g)分別為SEQ ID NOs:31、36及44;h)分別為SEQ ID NOs: 31、36及45;i)分別為SEQ ID NOs: 31、36及46;j)分別為SEQ ID NOs: 32、41及47;或k)分別為SEQ ID NOs: 33、41及48。The invention also relates to a humanized immunoglobulin light chain of a humanized immunoglobulin as described herein. In one embodiment, the humanized immunoglobulin light chain comprises SEQ ID NO:27, SEQ ID NO:28, SEQ ID NO:29, SEQ ID NO:30, SEQ ID NO:31, SEQ ID NO:32 SEQ ID NO: 33, SEQ ID NO: 34, SEQ ID NO: 35, SEQ ID NO: 36, SEQ ID NO: 37, SEQ ID NO: 38, SEQ ID NO: 39, SEQ ID NO: 40, SEQ ID NO:41, SEQ ID NO:42, SEQ ID NO:43, SEQ ID NO:44, SEQ ID NO:45, SEQ ID NO:46, SEQ ID NO:47, and SEQ ID NO:48 One or more selected CDRs, and combinations thereof, wherein the humanized immunoglobulin light chain is not Campath Light chain. For example, the humanized antibody has the amino acid sequence of L-CDR1, L-CDR2 and L-CDR3: a) SEQ ID NOs: 29, 36 and 43; b) SEQ ID NOs: 29, 37 and 43; c) SEQ ID NOs: 29, 38 and 43; d) SEQ ID NOs: 29, 36 and 43, respectively; e) SEQ ID NOs: 29, 39 and 43; f) SEQ ID, respectively NOs: 30, 40, and 43; g) are SEQ ID NOs: 31, 36, and 44; h) are SEQ ID NOs: 31, 36, and 45, respectively; i) are SEQ ID NOs: 31, 36, and 46, respectively; j) SEQ ID NOs: 32, 41 and 47; or k) are SEQ ID NOs: 33, 41 and 48, respectively.

本發明亦相關於一種人類化重鏈,其包含由SEQ ID NO: 49、SEQ ID NO: 50、SEQ ID NO: 51、SEQ ID NO:52、SEQ ID NO:53、SEQ ID NO: 54、SEQ ID NO: 55、SEQ ID NO: 56、SEQ ID NO:57、SEQ ID NO:58、SEQ ID NO:59、SEQ ID NO:60、SEQ ID NO:61、SEQ ID NO:62、SEQ ID NO:63、SEQ ID NO:64、SEQ ID NO:65、SEQ ID NO:66、SEQ ID NO:67、SEQ ID NO: 68、SEQ ID NO:69、SEQ ID NO:70、SEQ ID NO:71、SEQ ID NO:72、SEQ ID NO:73、SEQ ID NO:74及SEQ ID NO:294所組成族群選出的一或多個CDR,或是其組合,其中該人類化免疫球蛋白重鏈不為Campath的重鏈。例如,該人類化抗體具H-CDR1、H-CDR2、及H-CDR3其胺基酸序列:a).分別為SEQ ID NOs: 51、59及69;b)分別為SEQ ID NOs: 50、60及69;c)分別為SEQ ID NOs: 50、61及68;d)分別為SEQ ID NOs: 50、61及69;e)分別為SEQ ID NOs: 50、62及69;f)分別為SEQ ID NOs: 52、61及70;g)分別為SEQ ID NOs: 53、63、及71;h)分別為SEQ ID NOs: 54、64及71;i)分別為SEQ ID NOs: 55、63及72;j)分別為SEQ ID NOs: 56、65及73;k)分別為SEQ ID NOs: 56、65及294;或1)分別為SEQ ID NOs: 56、66及74。The invention also relates to a humanized heavy chain comprising SEQ ID NO: 49, SEQ ID NO: 50, SEQ ID NO: 51, SEQ ID NO: 52, SEQ ID NO: 53, SEQ ID NO: 54, SEQ ID NO: 55, SEQ ID NO: 56, SEQ ID NO: 57, SEQ ID NO: 58, SEQ ID NO: 59, SEQ ID NO: 60, SEQ ID NO: 61, SEQ ID NO: 62, SEQ ID NO: 63, SEQ ID NO: 64, SEQ ID NO: 65, SEQ ID NO: 66, SEQ ID NO: 67, SEQ ID NO: 68, SEQ ID NO: 69, SEQ ID NO: 70, SEQ ID NO: 71. One or more CDRs selected from the group consisting of SEQ ID NO: 72, SEQ ID NO: 73, SEQ ID NO: 74, and SEQ ID NO: 294, or a combination thereof, wherein the humanized immunoglobulin heavy chain Not for Campath Heavy chain. For example, the humanized antibody has the amino acid sequence of H-CDR1, H-CDR2, and H-CDR3: a). SEQ ID NOs: 51, 59, and 69; b) SEQ ID NOs: 50, respectively. 60 and 69; c) SEQ ID NOs: 50, 61 and 68; d) SEQ ID NOs: 50, 61 and 69; e) SEQ ID NOs: 50, 62 and 69, respectively; f) And SEQ ID NOs: 53, 63, and 71; And 72; j) are SEQ ID NOs: 56, 65 and 73; k) are SEQ ID NOs: 56, 65 and 294, respectively; or 1) are SEQ ID NOs: 56, 66 and 74, respectively.

在一個實施例中,本發明人類化抗體包含一種輕鏈,其包含SEQ ID NOs: 102、138、145-148、153-157及164-168其中一個的變異區(VL)序列。在相關實施例中,該人類化抗體包含一種輕鏈,其胺基酸序列包含或由SEQ ID NOs: 273、275、278、280及282其中之一組成。In one embodiment, the humanized antibody of the present invention comprises one light chain which comprises SEQ ID NOs: 102,138,145-148,153-157 and 164-168 wherein a variable region of (V L) sequence. In a related embodiment, the humanized antibody comprises a light chain comprising an amino acid sequence consisting of or consisting of one of SEQ ID NOs: 273, 275, 278, 280 and 282.

在一個具體實施例,本發明人類化抗體包含一種重鏈,其包含SEQ ID NOs: 103、136、137、139-144、149-152及158-163其中一個的變異區(VH)序列。在相關具體實施例,該人類化抗體包含一種輕鏈,其胺基酸序列包含SEQ ID NOs: 272、274、276、277、279及281其中一個或由之組成。In a specific embodiment, the humanized antibody of the invention comprises a heavy chain comprising a variant region ( VH ) sequence of one of SEQ ID NOs: 103, 136, 137, 139-144, 149-152, and 158-163. In a related embodiment, the humanized antibody comprises a light chain, the amino acid sequence comprising or consisting of one of SEQ ID NOs: 272, 274, 276, 277, 279 and 281.

在一些具體實施例,本發明人類化抗體包含VH及VL,其胺基酸序列包含或由下列組成In some embodiments, humanized antibodies of the invention comprise V H and V L, which amino acid sequence comprises or consists of

a) 分別為SEQ ID NOs: 103及102(4B10-H1/K1);a) are SEQ ID NOs: 103 and 102, respectively (4B10-H1/K1);

b) 分別為SEQ ID NOs: 136及138(7F11-SFD1/K2);b) are SEQ ID NOs: 136 and 138, respectively (7F11-SFD1/K2);

c) 分別為SEQ ID NOs: 137及138(7F11-SFD2/K2);c) are SEQ ID NOs: 137 and 138, respectively (7F11-SFD2/K2);

d) 分別為SEQ ID NO: 139及SEQ ID NOs: 145-148其中一個(例如,分別為SEQ ID NOs: 139及146(2C3-SFD1/K11);及分別為SEQ ID NOs: 139及147(2C3-SFD1/K12)):d) one of SEQ ID NO: 139 and SEQ ID NOs: 145-148, respectively (eg, SEQ ID NOs: 139 and 146 (2C3-SFD1/K11), respectively; and SEQ ID NOs: 139 and 147, respectively ( 2C3-SFD1/K12)):

e) 分別為SEQ ID NO: 140及SEQ ID NOs: 145-148其中一個;e) one of SEQ ID NO: 140 and SEQ ID NOs: 145-148, respectively;

f)分別為SEQ ID NO: 141及SEQ ID NOs: 145-148其中一個;f) one of SEQ ID NO: 141 and SEQ ID NOs: 145-148, respectively;

g)分別為SEQ ID NO: 142及SEQ ID NOs: 145-148其中一個;g) one of SEQ ID NO: 142 and SEQ ID NOs: 145-148, respectively;

h)分別為SEQ ID NO: 143及SEQ ID NOs: 145-148其中一個;h) one of SEQ ID NO: 143 and SEQ ID NOs: 145-148, respectively;

i)分別為SEQ ID NO: 144及SEQ ID NOs: 145-148其中一個;i) one of SEQ ID NO: 144 and SEQ ID NOs: 145-148, respectively;

j)分別為SEQ ID NO: 149及SEQ ID NOs: 153-157其中一個(例如,分別為SEQ ID NOs: 149及155(12G6-SFD1/K11);分別為SEQ ID NOs: 149及156(12G6-SFD1/K12);及分別為SEQ ID NOs: 149及157(12G6-SFD1/K13));j) one of SEQ ID NO: 149 and SEQ ID NOs: 153-157, respectively (eg, SEQ ID NOs: 149 and 155, respectively (12G6-SFD1/K11); SEQ ID NOs: 149 and 156 (12G6, respectively) -SFD1/K12); and SEQ ID NOs: 149 and 157 (12G6-SFD1/K13), respectively;

k)分別為SEQ ID NO: 150及SEQ ID NOs: 153-157其中一個;k) one of SEQ ID NO: 150 and SEQ ID NOs: 153-157, respectively;

l)分別為SEQ ID NO: 151及SEQ ID NOs: 153-157其中一個;l) one of SEQ ID NO: 151 and SEQ ID NOs: 153-157, respectively;

m)分別為SEQ ID NO: 152及SEQ ID NOs: 153-157其中一個;m) one of SEQ ID NO: 152 and SEQ ID NOs: 153-157, respectively;

n)分別為SEQ ID NO: 158及SEQ ID NOs: 164-168其中一個(例如,SEQ ID NOs: 158以及165(9D9-H10/K12);及SEQ ID NOs: 158及166(9D9-H10/K13));n) one of SEQ ID NO: 158 and SEQ ID NOs: 164-168, respectively (eg, SEQ ID NOs: 158 and 165 (9D9-H10/K12); and SEQ ID NOs: 158 and 166 (9D9-H10/) K13));

o)分別為SEQ ID NO: 159及SEQ ID NOs: 164-168其中一個(例如,SEQ ID NOs: 159及165(9D9-H11/K12);及SEQ ID NOs: 159及166(9D9-H11/K13));o) one of SEQ ID NO: 159 and SEQ ID NOs: 164-168, respectively (eg, SEQ ID NOs: 159 and 165 (9D9-H11/K12); and SEQ ID NOs: 159 and 166 (9D9-H11/) K13));

p) 分別為SEQ ID NO: 160及SEQ ID NOs: 164-168其中一個;p) one of SEQ ID NO: 160 and SEQ ID NOs: 164-168, respectively;

q) 分別為SEQ ID NO: 161及SEQ ID NOs: 164-168其中一個(例如,分別為SEQ ID NOs: 161及166(9D9-H16/K13));q) one of SEQ ID NO: 161 and SEQ ID NOs: 164-168, respectively (eg, SEQ ID NOs: 161 and 166 (9D9-H16/K13), respectively);

r) 分別為SEQ ID NO: 162及SEQ ID NOs: 164-168其中一個;或r) one of SEQ ID NO: 162 and SEQ ID NOs: 164-168, respectively; or

s) 分別為SEQ ID NO: 163及SEQ ID NOs: 164-168其中一個(例如,分別為SEQ ID NOs: 163及166(9D9-H18/K13))。s) are one of SEQ ID NO: 163 and SEQ ID NOs: 164-168, respectively (eg, SEQ ID NOs: 163 and 166, respectively (9D9-H18/K13)).

包含於括弧的抗體進一步於下列實例敘述。The antibodies contained in parentheses are further described in the following examples.

在一些具體實施例,本發明人類化抗體包含輕鏈(LC)及重鏈(HC),其胺基酸序列包含或由下列組成a)分別為SEQ ID NOs: 273及272;b)分別為SEQ ID NOs: 275及274;c)分別為SEQ ID NOs: 278及276;d)分別為SEQ ID NOs: 278及277;e)分別為SEQ ID NOs: 280及279;或f) 分別為SEQ ID NOs: 282及281。In some embodiments, the humanized antibodies of the invention comprise a light chain (LC) and a heavy chain (HC), the amino acid sequence of which comprises or consists of a) SEQ ID NOs: 273 and 272, respectively; b) And SEQ ID NOs: 278 and 276; ID NOs: 282 and 281.

本發明亦提供一種抗-人類CD52抗體(除了在先前技藝中已知的那些),其結合至與此處所示例抗體相同的抗原決定區,或是與之競爭或交互競爭。這些抗體可為,例如,人類化、嵌合、或老鼠抗體。例如,本發明提供一種抗-人類CD52抗體,其結合至與老鼠抗體8G3、4F7、9D9、11C11、3G7、5F7、12G6、23E6、2C3、7F11及4B10及這些老鼠抗體的人類化及嵌合抗體其中一個相同的抗原決定區,或是與之競爭或交互競爭。抗體結合至與參考抗體相同的抗原決定區,或是與之競爭或交互競爭之能力可如上文所敘述決定,例如,我們發現由人類化抗體2C3-SFD1/K12及12G6-SFD1/K12所結合的CD52抗原決定區包含於SEQ ID NO:104的殘基7、8、及11,及由人類化抗體9D9-H16/K13所結合的抗原決定區包含於SEQ ID NO:104的殘基4及11。於是,在一些具體實施例,本發明提供一種抗-CD52抗體,其結合至與那些人類化抗體相同的抗原決定區,或是與之競爭或交互競爭。The invention also provides an anti-human CD52 antibody (other than those known in the prior art) that binds to, competes with or competes with, the same epitope as the antibodies set forth herein. These antibodies can be, for example, humanized, chimeric, or mouse antibodies. For example, the present invention provides an anti-human CD52 antibody which binds to mouse antibodies 8G3, 4F7, 9D9, 11C11, 3G7, 5F7, 12G6, 23E6, 2C3, 7F11 and 4B10 and humanized and chimeric antibodies of these mouse antibodies One of the same epitopes, either competing or competing with it. The ability of an antibody to bind to, or compete with, the same epitope as the reference antibody can be determined as described above. For example, we found that the humanized antibody 2C3-SFD1/K12 and 12G6-SFD1/K12 are combined. The CD52 epitope is contained in residues 7, 8, and 11 of SEQ ID NO: 104, and the epitope determined by the humanized antibody 9D9-H16/K13 is contained in residue 4 of SEQ ID NO: 104 and 11. Thus, in some embodiments, the invention provides an anti-CD52 antibody that binds to, or competes with, or competes with the same epitope of those humanized antibodies.

若希望,例如,為診斷或試驗目的(例如,使可醫療監控),人類化免疫球蛋白(例如,其抗原-結合片段)可包含可偵測標記,合適的可偵測標記及人類化免疫球蛋白或其抗原-結合片段的標記方法為該技藝已知。合適的可偵測標記包含,例如,放射性同位素(例如,銦-111、鍀-99m或碘-131)、正子放射型標記(例如,氟-19)、順磁離子(例如,釓(III)、錳(II))、抗原決定區標記(標籤)、親和性標記(例如,生物素、卵白素)、自旋標記、酶、螢光族群或化學發光族群。當未使用標記時,複合物形成(例如,在人類化免疫球蛋白及人類CD52之間)可由表面電漿共振、ELISA、FACS、或其他合適方法決定。If desired, for example, for diagnostic or experimental purposes (eg, for medical monitoring), humanized immunoglobulins (eg, antigen-binding fragments thereof) can include detectable labels, suitable detectable labels, and humanized immunity. Methods of labeling globulin or antigen-binding fragments thereof are known in the art. Suitable detectable labels include, for example, radioisotopes (eg, indium-111, yttrium-99m or iodine-131), positron-type labels (eg, fluorine-19), paramagnetic ions (eg, ruthenium (III)) , manganese (II)), epitope (tag), affinity tag (eg, biotin, avidin), spin label, enzyme, fluorescent population, or chemiluminescent population. When no label is used, complex formation (eg, between humanized immunoglobulin and human CD52) can be determined by surface plasma resonance, ELISA, FACS, or other suitable method.

用於本發明的抗-CD52抗體亦可經由例如,化學反應或基因修飾而共軛至其他基團(例如,聚乙二醇化聚基團),上述基團改善抗體的藥物動力,例如半衰期。在一些具體實施例,用於本發明的抗-CD52抗體可經由例如,化學共軛或基因修飾(例如,附加骨架中細胞介素編碼序列至抗體編碼序列,由此產生抗體:細胞介素融合蛋白)而連結至合適細胞介素。Anti-CD52 antibodies useful in the present invention may also be conjugated to other groups (e.g., PEGylated poly groups) via, for example, chemical reactions or genetic modifications that improve the drug motility, e.g., half-life, of the antibody. In some embodiments, an anti-CD52 antibody for use in the present invention can be produced, for example, by chemical conjugation or genetic modification (eg, an additional intervening interleukin coding sequence to an antibody coding sequence, thereby producing an antibody: interleukin fusion Protein) and linked to a suitable interleukin.

本發明亦關於一種免疫接合,其中本發明的人類化免疫球蛋白(例如,其抗原-結合片段)係耦合至另一醫療劑,例如生物活性化合物(例如,細胞介素、超抗原、細胞毒性化療劑及毒素)。例如,具對人類CD52結合專一性的人類化免疫球蛋白(例如,其抗原-結合片段)可耦合至生物蛋白,一種植物或細菌來源的分子(或其衍生物)、白血球介素-2抗體或白喉毒素抗體。The invention also relates to an immunological junction wherein the humanized immunoglobulin of the invention (eg, an antigen-binding fragment thereof) is linked to another medical agent, such as a biologically active compound (eg, interleukin, superantigen, cytotoxicity) Chemotherapeutic agents and toxins). For example, a humanized immunoglobulin (eg, an antigen-binding fragment thereof) that binds to human CD52 binding can be coupled to a biological protein, a plant or bacterial derived molecule (or derivative thereof), a white blood interleukin-2 antibody Or diphtheria toxin antibody.

老鼠單株免疫球蛋白Mouse monoclonal immunoglobulin

如此處所敘述,本發明已製造出具有對人類CD52結合專一性的老鼠單株免疫球蛋白。本發明的人類化及嵌合抗體可衍生自本發明老鼠單株免疫球蛋白。亦即,在一些具體實施例,本發明的人類化及嵌合抗-CD52抗體包含取自本發明老鼠單株抗體的序列,例如一或更多CDR序列。本發明的老鼠單株免疫球蛋白包含具有與已知老鼠抗-CD52單株抗體的CDR胺基酸序列不同的CDR胺基酸序列的輕鏈及重鏈(例如,得自CF1D12)。As described herein, the present invention has produced mouse monoclonal immunoglobulins having specificity for human CD52 binding. The humanized and chimeric antibodies of the invention can be derived from the mouse monoclonal immunoglobulin of the invention. That is, in some embodiments, the humanized and chimeric anti-CD52 antibodies of the invention comprise sequences derived from a mouse monoclonal antibody of the invention, such as one or more CDR sequences. The mouse monoclonal immunoglobulin of the present invention comprises a light chain and a heavy chain (for example, obtained from CF1D12) having a CDR amino acid sequence different from the CDR amino acid sequence of a known mouse anti-CD52 monoclonal antibody.

當用於此處時,名稱「老鼠單株免疫球蛋白」係表示一種包含老鼠抗-人類CD52抗體的輕鏈CDRs(L-CDR1、L-CDR2及L-CDR3)及重鏈CDRs(H-CDR1、H-CDR2及H-CDR3),及老鼠來源的骨架及恆定區的免疫球蛋白。老鼠單株免疫球蛋白為一種例如由使用融合瘤細胞計數法或重組方法所製備的單一專一性之同源抗體。As used herein, the designation "mouse monoclonal immunoglobulin" refers to a light chain CDR (L-CDR1, L-CDR2 and L-CDR3) and heavy chain CDRs (H-) comprising a mouse anti-human CD52 antibody. CDR1, H-CDR2 and H-CDR3), and mouse-derived backbone and constant region immunoglobulins. The mouse monoclonal immunoglobulin is a single specific homologous antibody prepared, for example, by using fusion tumor cell counting or recombinant methods.

本發明係關於一種此處所敘述老鼠單株免疫球蛋白,其包含老鼠單株免疫球蛋白的抗原-結合片段(亦即,部分)、老鼠單株免疫球蛋白的輕鏈、老鼠單株免疫球蛋白的重鏈、及重鏈及輕鏈的片段。在特別具體實施例,老鼠單株免疫球蛋白為老鼠8G3.25.3.5(亦稱為GENZ 8G3.25.3.5或8G3)、老鼠GMA 4G7.F3(亦稱為4G7.F3或4G7)、老鼠GMA 9D9.A2(亦稱為9D9.A2或9D9)、老鼠GMA 11C11.C5(亦稱為11C11.C5或11C11)、老鼠GMA 3G7.E9(亦稱為3G7.E9或3G7)、老鼠5F7.1.1.4(亦稱為GENZ 5F7.1.1.4或5F7)、老鼠12G6.15.1.2(亦稱為GENZ 12G6.15.1.2或2G6)、老鼠23E6.2.2.1(亦稱為GENZ 23E6.2.2.1或23E6)、老鼠2C3.3.8.1(亦稱為GENZ 2C3.3.8.1或2C3)、老鼠7F11.1.9.7(亦稱為GENZ 7F11.1.9.7或7F11)、或是老鼠4B10.1.2.4(亦稱為GENZ 4B10.1.2.4或4B10)。本發明係關於一種成熟老鼠單株免疫球蛋白,例如接著進行移除重鏈及輕鏈信號胜肽的老鼠單株免疫球蛋白及/或關於醣化免疫球蛋白。本發明亦關於一種不成熟或前驅蛋白質,例如包含信號胜肽的老鼠免疫球蛋白輕鏈或老鼠免疫球蛋白重鏈。本發明亦關於一種編碼這些不成熟或成熟蛋白的核酸分子(例如,載體),關於包含此種核酸的宿主細胞及關於這些不成熟及成熟蛋白的製造方法。The present invention relates to a mouse monoclonal immunoglobulin as described herein, which comprises an antigen-binding fragment (ie, a part) of a mouse monoclonal immunoglobulin, a light chain of a mouse monoclonal immunoglobulin, and a mouse monoclonal immunoglobulin. Heavy chain of protein, and fragments of heavy and light chains. In a specific embodiment, the mouse monoclonal immunoglobulin is mouse 8G3.25.3.5 (also known as GENZ 8G3.25.3.5 or 8G3), mouse GMA 4G7.F3 (also known as 4G7.F3 or 4G7), mouse GMA 9D9.A2 (also known as 9D9.A2 or 9D9), mouse GMA 11C11.C5 (also known as 11C11.C5 or 11C11), mouse GMA 3G7.E9 (also known as 3G7.E9 or 3G7), mouse 5F7. 1.1.4 (also known as GENZ 5F7.1.1.4 or 5F7), mouse 12G6.15.1.2 (also known as GENZ 12G6.15.1.2 or 2G6), mouse 23E6.2.2.1 (also known as GENZ 23E6. 2.2.1 or 23E6), mouse 2C3.3.8.1 (also known as GENZ 2C3.3.8.1 or 2C3), mouse 7F11.1.9.7 (also known as GENZ 7F11.1.9.7 or 7F11), or mouse 4B10.1.2.4 (also known as GENZ 4B10.1.2.4 or 4B10). The present invention relates to a mature mouse monoclonal immunoglobulin, such as a mouse monoclonal immunoglobulin followed by removal of heavy and light chain signal peptides and/or for glycated immunoglobulin. The invention also relates to an immature or precursor protein, such as a mouse immunoglobulin light chain or a mouse immunoglobulin heavy chain comprising a signal peptide. The invention also relates to a nucleic acid molecule (e.g., vector) encoding such immature or mature proteins, to host cells comprising such nucleic acids, and to methods of making such immature and mature proteins.

具人類CD52結合專一性的老鼠單株免疫球蛋白之結合功能可使用任何合適方法偵測,例如,使用監控老鼠單株免疫球蛋白與人類CD52(例如,包含人類CD52的膜部分,或攜帶人類CD52的細胞,例如人類T細胞、人類B細胞、包含編碼人類CD52的核酸之CHO細胞或重組宿主細胞;具CD52胺基酸序列的肽(例如,合成肽))之間複合物的形成之試驗。The binding function of mouse monoclonal immunoglobulin with human CD52 binding specificity can be detected by any suitable method, for example, monitoring mouse monoclonal immunoglobulin and human CD52 (for example, a membrane portion containing human CD52, or carrying humans) Test for formation of complexes between cells of CD52, such as human T cells, human B cells, CHO cells or recombinant host cells comprising a nucleic acid encoding human CD52; peptides having a CD52 amino acid sequence (eg, synthetic peptides) .

此處亦提供老鼠免疫球蛋白的部份,其包含輕鏈、重鏈及輕及重鏈部份。這些免疫球蛋白部份可得自或衍生自免疫球蛋白(例如,藉由還原及/或裂解),或是編碼具有所欲性質(例如,結合人類CD52,序列類似性)的一部份免疫球蛋白或其鏈的核酸可被製造或表現,它們可由例如相關部份的重新合成所製備。包含老鼠來源所欲部份(例如,抗原-結合區域、CDR、FR、及/或C區域)的老鼠單株免疫球蛋白可使用合成及/或重組核酸製造以製備編碼所欲單株免疫球蛋白鏈的構成物(例如,cDNA)。為製備一部份鏈,可於所欲位置引入一或更多中止密碼子。編碼信號胜肽的序列亦可併入核酸(例如於合成時,於插入載體時),若天然信號胜肽序列為無法提供的,可使用來自其他抗體的信號胜肽序列(參看例如Kettleborough,C.A.,Protein Engineering 4:773-783(1991))。使用這些方法,此處所敘述方法或其他合適方法,可以很容易製造出變異物。Also provided herein are portions of the mouse immunoglobulin comprising a light chain, a heavy chain, and light and heavy chain portions. These immunoglobulin moieties can be obtained or derived from immunoglobulins ( eg, by reduction and/or cleavage), or can be encoded as part of a desired property (eg, binding to human CD52, sequence similarity). Nucleic acids of globulin or its chains can be made or expressed, and they can be prepared, for example, by resynthesis of related moieties. Mouse monoclonal immunoglobulins containing portions of the mouse source (eg, antigen-binding regions, CDRs, FRs, and/or C regions) can be made using synthetic and/or recombinant nucleic acids to prepare immunoglobulins encoding the desired individual antibodies. A construct of a protein chain ( for example, cDNA). To prepare a portion of the strand, one or more stop codons can be introduced at the desired position. The sequence encoding the signal peptide can also be incorporated into the nucleic acid (eg , upon insertion into the vector), and if the native signal peptide sequence is not available, a signal peptide sequence from other antibodies can be used (see, eg , Kettleborough). , CA, Protein Engineering 4: 773-783 (1991)). Variants can be readily produced using these methods, methods described herein, or other suitable methods.

在一個具體實施例,本發明老鼠單株免疫球蛋白包含由SEQ ID NO:3組成的輕鏈及由SEQ ID NO:16組成的重鏈;由SEQ ID NO:4組成的輕鏈及由SEQ ID NO:17組成的重鏈;由SEQ ID NO:5組成的輕鏈及由SEQ ID NO:18組成的重鏈;由SEQ ID NO:6組成的輕鏈及由SEQ ID NO:19組成的重鏈;由SEQ ID NO:7組成的輕鏈及由SEQ ID NO:20組成的重鏈;由SEQ ID NO:8組成的輕鏈及由SEQ ID NO:21組成的重鏈;由SEQ ID NO:9組成的輕鏈及由SEQ ID NO:22組成的重鏈;由SEQ ID NO:10組成的輕鏈及由SEQ ID NO:23組成的重鏈;由SEQ ID NO:11組成的輕鏈及由SEQ ID NO:24組成的重鏈;由SEQ ID NO:12組成的輕鏈及由SEQ ID NO:25組成的重鏈;或由SEQ ID NO:13組成的輕鏈及由SEQ ID NO:26組成的重鏈。In a specific embodiment, the mouse monoclonal immunoglobulin of the invention comprises a light chain consisting of SEQ ID NO: 3 and a heavy chain consisting of SEQ ID NO: 16; a light chain consisting of SEQ ID NO: 4 and SEQ ID NO: heavy chain consisting of 17; a light chain consisting of SEQ ID NO: 5 and a heavy chain consisting of SEQ ID NO: 18; a light chain consisting of SEQ ID NO: 6 and consisting of SEQ ID NO: a heavy chain; a light chain consisting of SEQ ID NO: 7 and a heavy chain consisting of SEQ ID NO: 20; a light chain consisting of SEQ ID NO: 8 and a heavy chain consisting of SEQ ID NO: 21; NO: a light chain consisting of 9 and a heavy chain consisting of SEQ ID NO: 22; a light chain consisting of SEQ ID NO: 10 and a heavy chain consisting of SEQ ID NO: 23; light consisting of SEQ ID NO: a chain and a heavy chain consisting of SEQ ID NO: 24; a light chain consisting of SEQ ID NO: 12 and a heavy chain consisting of SEQ ID NO: 25; or a light chain consisting of SEQ ID NO: 13 and SEQ ID NO: Heavy chain consisting of 26.

在另一具體實施例,本發明亦關於一種具人類CD52結合專一性的老鼠單株抗體,其包含由SEQ ID NO:3、SEQ ID NO:4、SEQ ID NO:5、SEQ ID NO:6、SEQ ID NO:7、SEQ ID NO:8、SEQ ID NO:9、SEQ ID NO:10、SEQ ID NO:11、SEQ ID NO:12及SEQ ID NO:13所組成族群選出的輕鏈變異區;及由SEQ ID NO:16、SEQ ID NO:17、SEQ ID NO:18、SEQ ID NO:19、SEQ ID NO:20、SEQ ID NO:21、SEQ ID NO:22、SEQ ID NO:23、SEQ ID NO:24、SEQ ID NO:25及SEQ ID NO:26所組成族群選出的重鏈變異區。In another embodiment, the invention also relates to a mouse monoclonal antibody having human CD52 binding specificity comprising SEQ ID NO: 3, SEQ ID NO: 4, SEQ ID NO: 5, SEQ ID NO: 6. Light chain variation selected from the group consisting of SEQ ID NO: 7, SEQ ID NO: 8, SEQ ID NO: 9, SEQ ID NO: 10, SEQ ID NO: 11, SEQ ID NO: 12, and SEQ ID NO: And SEQ ID NO: 16, SEQ ID NO: 17, SEQ ID NO: 18, SEQ ID NO: 19, SEQ ID NO: 20, SEQ ID NO: 21, SEQ ID NO: 22, SEQ ID NO: 23. A heavy chain variant region selected from the group consisting of SEQ ID NO: 24, SEQ ID NO: 25 and SEQ ID NO: 26.

若希望,例如,為診斷或試驗目的(例如,想像),老鼠單株免疫球蛋白(例如,其抗原-結合片段)可包含可偵測標記,合適的可偵測標記及老鼠單株免疫球蛋白的標記方法為該技藝已知。合適的可偵測標記包含,例如,放射性同位素(例如,銦-111、鍀-99m或碘-131)、正子放射型標記(例如,氟-19)、順磁離子(例如,釓(III)、錳(II))、抗原決定區標記(標籤)、親和性標記(例如,生物素、卵白素)、自旋標記、酶、螢光族群或化學發光族群。當未使用標記時,複合物形成(例如,在老鼠單株免疫球蛋白及CD52之間)可由表面電漿共振或其他合適方法決定。上文針對本發明人類化抗體所敘述的所有合適方法及技術可於此處使用。If desired, for example, for diagnostic or experimental purposes (eg, imagining), a mouse monoclonal immunoglobulin (eg, an antigen-binding fragment thereof) can comprise a detectable marker, a suitable detectable marker, and a mouse immunoglobulin Methods of labeling proteins are known in the art. Suitable detectable labels include, for example, radioisotopes (eg, indium-111, yttrium-99m or iodine-131), positron-type labels (eg, fluorine-19), paramagnetic ions (eg, ruthenium (III)) , manganese (II)), epitope (tag), affinity tag (eg, biotin, avidin), spin label, enzyme, fluorescent population, or chemiluminescent population. When no label is used, complex formation (e.g., between mouse monoclonal immunoglobulin and CD52) can be determined by surface plasma resonance or other suitable method. All suitable methods and techniques described above for the humanized antibodies of the invention can be used herein.

嵌合免疫球蛋白Chimeric immunoglobulin

如此處所敘述,已製造具對人類CD52結合專一性的嵌合免疫球蛋白。嵌合免疫球蛋白包含嵌合輕鏈及/或嵌合重鏈,其胺基酸序列不同於具有對人類CD52結合專一性的已知嵌合抗體的胺基酸序列的。As described herein, chimeric immunoglobulins that have specificity for human CD52 binding have been made. Chimeric immunoglobulins comprise a chimeric light chain and/or a chimeric heavy chain, the amino acid sequence of which differs from the amino acid sequence of a known chimeric antibody having specificity for human CD52 binding.

當用於此處時,名稱「嵌合免疫球蛋白」係表示一種重組蛋白,其包含含有衍生自一種物種的抗體,較佳為老鼠抗-人類CD52單株抗體的互補決定區段(CDRs)的變異區,然而抗體分子的恆定區係得自不同物種,例如人類抗體。As used herein, the term "chimeric immunoglobulin" refers to a recombinant protein comprising complementarity determining regions (CDRs) comprising antibodies derived from a species, preferably mouse anti-human CD52 monoclonal antibodies. The variant region, however, the constant region of the antibody molecule is derived from a different species, such as a human antibody.

本發明係關於此處所敘述嵌合免疫球蛋白,其包含嵌合免疫球蛋白的抗原-結合片段(亦即,部分)、嵌合免疫球蛋白的嵌合輕鏈及嵌合重鏈及這些嵌合輕及重鏈的片段。本發明係關於一種成熟嵌合免疫球蛋白,例如接著進行移除重鏈及輕鏈信號胜肽的嵌合免疫球蛋白及/或關於醣化免疫球蛋白。本發明亦關於一種不成熟或前驅蛋白質,例如包含信號胜肽的嵌合重鏈。本發明亦關於一種編碼這些不成熟或成熟蛋白的核酸分子(例如,載體),關於包含此種核酸的宿主細胞及關於這些不成熟及成熟蛋白的製造方法。The present invention relates to a chimeric immunoglobulin as described herein, which comprises an antigen-binding fragment (i.e., a portion) of a chimeric immunoglobulin, a chimeric light chain of a chimeric immunoglobulin, and a chimeric heavy chain, and these inlays Fragments of light and heavy chains. The present invention relates to a mature chimeric immunoglobulin, such as a chimeric immunoglobulin followed by removal of a heavy chain and a light chain signal peptide and/or to a glycosylated immunoglobulin. The invention also relates to an immature or precursor protein, such as a chimeric heavy chain comprising a signal peptide. The invention also relates to a nucleic acid molecule (e.g., vector) encoding such immature or mature proteins, to host cells comprising such nucleic acids, and to methods of making such immature and mature proteins.

具有人類CD52結合專一性的嵌合免疫球蛋白之結合功能可使用任何合適方法偵測,例如使用監控嵌合免疫球蛋白與人類CD52(例如,包含人類CD52的膜部分,或攜帶人類CD52的細胞,例如人類T細胞、人類B細胞、CHO細胞或包含編碼人類CD52的核酸之重組宿主細胞;具CD52胺基酸序列的肽(例如,合成肽))之間複合物的形成之試驗。The binding function of a chimeric immunoglobulin having human CD52 binding specificity can be detected using any suitable method, for example, using a chimeric immunoglobulin to monitor human CD52 (eg, a membrane portion comprising human CD52, or a cell carrying human CD52). An assay for the formation of a complex between, for example, a human T cell, a human B cell, a CHO cell, or a recombinant host cell comprising a nucleic acid encoding human CD52; a peptide having a CD52 amino acid sequence (eg, a synthetic peptide).

此處亦提供的是嵌合免疫球蛋白的部份,其包含輕鏈、重鏈及輕與重鏈的部份。這些免疫球蛋白部份可得自或衍生自免疫球蛋白(例如藉由還原及/或裂解),或是編碼具有所欲性質(例如,結合人類CD52,序列類似性)的一部份免疫球蛋白或其鏈的核酸可被製造或表現,它們可由例如相關部份的重新合成所製備。包含人類及非人類來源所欲部份(例如,抗原-結合區域、CDR、FR、及/或C區域)的嵌合免疫球蛋白可使用合成及/或重組核酸製造以製備編碼所欲嵌合鏈的構成物(例如cDNA)。為製備一部份鏈,可於所欲位置引入一或更多中止密碼子。編碼信號胜肽的序列亦可併入核酸(例如,於合成時,於插入載體時),若天然信號胜肽序列為無法提供的(例如,典型上不存在),可使用來自其他抗體的信號胜肽序列(參看例如,Kettleborough,C.A.,Protein Engineering 4:773-783(1991))。使用這些方法,此處所敘述方法或其他合適方法,可以容易地製造出變異物。Also provided herein are portions of chimeric immunoglobulins comprising a light chain, a heavy chain, and a light and heavy chain portion. These immunoglobulin moieties can be obtained or derived from immunoglobulins (eg , by reduction and/or cleavage), or can be encoded as part of a desired property (eg, binding to human CD52, sequence similarity). Nucleic acids of globulin or its chains can be made or expressed, and they can be prepared, for example, by resynthesis of related moieties. Chimeric immunoglobulins comprising portions of human and non-human origin (eg, antigen-binding regions, CDRs, FRs, and/or C regions) can be made using synthetic and/or recombinant nucleic acids to prepare the desired coding The composition of the strand (for example , cDNA). To prepare a portion of the strand, one or more stop codons can be introduced at the desired position. The sequence encoding the signal peptide can also be incorporated into the nucleic acid ( eg, upon insertion into the vector), and if the native signal peptide sequence is not available (eg, typically not present), signals from other antibodies can be used. The peptide sequence (see, for example, Kettleborough, CA, Protein Engineering 4:773-783 (1991)). Variants can be readily produced using these methods, methods described herein, or other suitable methods.

在一個具體實施例,本發明嵌合免疫球蛋白包含SEQ ID NO: 3的輕鏈變異區及SEQ ID NO: 16的重鏈變異區;SEQ ID NO: 4的輕鏈變異區及SEQ ID NO: 17的重鏈變異區;SEQ ID NO: 5的輕鏈變異區及SEQ ID NO: 18的重鏈變異區;SEQ ID NO: 6的輕鏈變異區及SEQ ID NO: 19的重鏈變異區;SEQ ID NO: 7的輕鏈變異區及SEQ ID NO: 20的重鏈變異區;SEQ ID NO: 8的輕鏈變異區及SEQ ID NO: 21的重鏈變異區;SEQ ID NO: 9的輕鏈變異區及SEQ ID NO: 22的重鏈變異區;SEQ ID NO: 10的輕鏈變異區及SEQ ID NO: 23的重鏈變異區;SEQ ID NO: 11的輕鏈變異區及SEQ ID NO: 24的重鏈變異區;SEQ ID NO: 12的輕鏈變異區及SEQ ID NO: 25的重鏈變異區;或是SEQ ID NO: 13的輕鏈變異區及SEQ ID NO: 26的重鏈變異區。In a specific embodiment, the chimeric immunoglobulin of the invention comprises the light chain variant region of SEQ ID NO: 3 and the heavy chain variant region of SEQ ID NO: 16; the light chain variant region of SEQ ID NO: 4 and SEQ ID NO : a heavy chain variant region of 17; a light chain variant region of SEQ ID NO: 5 and a heavy chain variant region of SEQ ID NO: 18; a light chain variant region of SEQ ID NO: 6 and a heavy chain variant of SEQ ID NO: Region; the light chain variant region of SEQ ID NO: 7 and the heavy chain variant region of SEQ ID NO: 20; the light chain variant region of SEQ ID NO: 8 and the heavy chain variant region of SEQ ID NO: 21; SEQ ID NO: a light chain variant region of 9 and a heavy chain variant region of SEQ ID NO: 22; a light chain variant region of SEQ ID NO: 10 and a heavy chain variant region of SEQ ID NO: 23; a light chain variant region of SEQ ID NO: And the heavy chain variant region of SEQ ID NO: 24; the light chain variant region of SEQ ID NO: 12 and the heavy chain variant region of SEQ ID NO: 25; or the light chain variant region of SEQ ID NO: 13 and SEQ ID NO : 26 heavy chain variation regions.

本發明亦關於一種具對人類CD52的結合專一性的嵌合抗體,其包含由下列所組成族群選出的輕鏈變異區序列:SEQ ID NO: 3的輕鏈變異區、SEQ ID NO: 4的輕鏈變異區、SEQ ID NO: 5的輕鏈變異區、SEQ ID NO: 6的輕鏈變異區、SEQ ID NO: 7的輕鏈變異區、SEQ ID NO: 8的輕鏈變異區、SEQ ID NO: 9的輕鏈變異區、SEQ ID NO: 10的輕鏈變異區、SEQ ID NO: 11的輕鏈變異區、SEQ ID NO: 12的輕鏈變異區及SEQ ID NO: 13的輕鏈變異區,及由下列所組成族群選出的重鏈變異區序列:SEQ ID NO: 16的重鏈變異區、SEQ ID NO: 17的重鏈變異區、SEQ ID NO: 18的重鏈變異區、SEQ ID NO: 19的重鏈變異區、SEQ ID NO: 20的重鏈變異區、SEQ ID NO: 21的重鏈變異區、SEQ ID NO: 22的重鏈變異區、SEQ ID NO: 23的重鏈變異區、SEQ ID NO: 24的重鏈變異區、SEQ ID NO: 25的重鏈變異區及SEQ ID NO: 26的重鏈變異區。The invention also relates to a chimeric antibody having binding specificity for human CD52 comprising a light chain variant region sequence selected from the group consisting of: the light chain variant region of SEQ ID NO: 3, SEQ ID NO: 4 a light chain variant region, a light chain variant region of SEQ ID NO: 5, a light chain variant region of SEQ ID NO: 6, a light chain variant region of SEQ ID NO: 7, a light chain variant region of SEQ ID NO: 8, SEQ ID NO: a light chain variant region of 9 , a light chain variant region of SEQ ID NO: 10, a light chain variant region of SEQ ID NO: 11, a light chain variant region of SEQ ID NO: 12, and a light SEQ ID NO: 13 a strand variant region, and a sequence of a heavy chain variant region selected from the group consisting of: a heavy chain variant region of SEQ ID NO: 16, a heavy chain variant region of SEQ ID NO: 17, and a heavy chain variant region of SEQ ID NO: 18. , the heavy chain variant region of SEQ ID NO: 19, the heavy chain variant region of SEQ ID NO: 20, the heavy chain variant region of SEQ ID NO: 21, the heavy chain variant region of SEQ ID NO: 22, SEQ ID NO: 23 The heavy chain variant region, the heavy chain variant region of SEQ ID NO: 24, the heavy chain variant region of SEQ ID NO: 25, and the heavy chain variant region of SEQ ID NO: 26.

本發明亦關於一種嵌合輕鏈,其包含SEQ ID NO: 3、SEQ ID NO: 4、SEQ ID NO: 5、SEQ ID NO: 6、SEQ ID NO: 7、SEQ ID NO: 8、SEQ ID NO: 9、SEQ ID NO: 10、SEQ ID NO: 11、SEQ ID NO: 12或SEQ ID NO: 13的變異區。The invention also relates to a chimeric light chain comprising SEQ ID NO: 3, SEQ ID NO: 4, SEQ ID NO: 5, SEQ ID NO: 6, SEQ ID NO: 7, SEQ ID NO: 8, SEQ ID NO: 9. The variant region of SEQ ID NO: 10, SEQ ID NO: 11, SEQ ID NO: 12 or SEQ ID NO: 13.

本發明亦關於一種嵌合重鏈,其包含SEQ ID NO:16、SEQ ID NO:17、SEQ ID NO:18、SEQ ID NO:19、SEQ ID NO:20、SEQ ID NO:21、SEQ ID NO:22、SEQ ID NO:23、SEQ ID NO:24、SEQ ID NO:25或SEQ ID NO:26的變異區。The invention also relates to a chimeric heavy chain comprising SEQ ID NO: 16, SEQ ID NO: 17, SEQ ID NO: 18, SEQ ID NO: 19, SEQ ID NO: 20, SEQ ID NO: 21, SEQ ID NO: 22, SEQ ID NO: 23, SEQ ID NO: 24, SEQ ID NO: 25 or the variant region of SEQ ID NO: 26.

若希望,例如,為診斷或試驗目的(例如,想像),嵌合免疫球蛋白(例如,其抗原-結合片段)可包含可偵測標記,合適的可偵測標記及嵌合免疫球蛋白或其抗原-結合片段的標記方法為該技藝已知。合適的可偵測標記包含,例如,放射性同位素(例如,銦-111、鍀-99m或碘-131)、正子放射型標記(例如,氟-19)、順磁離子(例如,釓(III)、錳(II))、抗原決定區標記(標籤)、親和性標記(例如,生物素、卵白素)、自旋標記、酶、螢光族群或化學發光族群。當未使用標記時,複合物形成(例如,在嵌合免疫球蛋白及人類CD52之間)可由表面電漿共振或其他合適方法決定。上文針對本發明人類化抗體所敘述的所有合適方法及技術可於此處使用。If desired, for example, for diagnostic or experimental purposes (eg, imagining), a chimeric immunoglobulin (eg, an antigen-binding fragment thereof) can comprise a detectable label, a suitable detectable label, and a chimeric immunoglobulin or Methods of labeling antigen-binding fragments thereof are known in the art. Suitable detectable labels include, for example, radioisotopes (eg, indium-111, yttrium-99m or iodine-131), positron-type labels (eg, fluorine-19), paramagnetic ions (eg, ruthenium (III)) , manganese (II)), epitope (tag), affinity tag (eg, biotin, avidin), spin label, enzyme, fluorescent population, or chemiluminescent population. When no label is used, complex formation (eg, between chimeric immunoglobulin and human CD52) can be determined by surface plasma resonance or other suitable method. All suitable methods and techniques described above for the humanized antibodies of the invention can be used herein.

核酸及重組載體Nucleic acid and recombinant vector

本發明亦關於一種經分離及/或重組(包含,例如,基本上純的)核酸,其包含編碼本發明人類化免疫球蛋白、人類化輕鏈、人類化重鏈、老鼠單株免疫球蛋白、老鼠免疫球蛋白輕鏈、老鼠免疫球蛋白重鏈、嵌合免疫球蛋白、嵌合輕鏈或嵌合重鏈的序列。The invention also relates to an isolated and/or recombinant (including, for example, substantially pure) nucleic acid comprising a humanized immunoglobulin encoding the invention, a humanized light chain, a humanized heavy chain, a mouse monoclonal immunoglobulin , a mouse immunoglobulin light chain, a mouse immunoglobulin heavy chain, a chimeric immunoglobulin, a chimeric light chain or a chimeric heavy chain.

此處稱為「分離」或"純化"的核酸為已分離自其起源(例如,當他們存在於細胞或於例如庫的核酸混合物)的基因體DNA或細胞RNA的核酸,及包含由此處所敘述方法或其他合適方法所得到的核酸,其包含大體上純的核酸,由化學合成,生物及化學方法的組合所分離重組核酸所製造的核酸(參考例如,Daugherty,B.L. et al.,Nucleic Acids Res.,19(9):2471-2476(1991);Lewis,A.P. and J.S. Crowe,Gene,101: 297-302(1991))。Nucleic acids referred to herein as "isolated" or "purified" are nucleic acids that have been isolated from the genomic DNA or cellular RNA of their origin (eg, when they are present in a cell or a mixture of nucleic acids, eg, a library), and are encompassed by A nucleic acid obtained by a narrative method or other suitable method, which comprises a substantially pure nucleic acid, a nucleic acid produced by separating a recombinant nucleic acid by a combination of chemical synthesis, biological and chemical methods (see, for example, Daugherty, BL et al., Nucleic Acids). Res., 19(9): 2471-2476 (1991); Lewis, AP and JS Crowe, Gene, 101: 297-302 (1991)).

此處稱為"重組"的核酸為重組DNA方法所製造的核酸,其包含由人工重組方法的步驟,例如聚合酶連鎖反應(PCR)及/或使用限制酵素選殖至載體所產生的核酸。"重組"核酸亦為那些得自在細胞自然機制過程發生的重組之核酸,但會被選擇以在引至核酸細胞之後,使所欲重組可發生。Nucleic acids referred to herein as "recombinant" are nucleic acids produced by recombinant DNA methods, which comprise steps by artificial recombination methods, such as polymerase chain reaction (PCR) and/or nucleic acid produced by confining enzymes to a vector. "Recombinant" nucleic acids are also those which are derived from recombinant processes occurring in the natural machinery of the cell, but which are selected to allow the desired recombination to occur after introduction to the nucleic acid cells.

本發明亦更特定地關於一種經分離及/或重組核酸,其包含編碼人類化免疫球蛋白、老鼠免疫球蛋白或嵌合免疫球蛋白的核苷酸序列,其具有對人類CD52的結合專一性(例如,一種本發明的人類化免疫球蛋白,其中非人類部份(例如,CDRs)係衍生自老鼠抗-CD52單株抗體;本發明的老鼠免疫球蛋白;或本發明的嵌合免疫球蛋白,其中非人類部份(例如,VH及VL)係衍生自老鼠抗-CD52單株抗體)或其部份(例如,抗原-結合部份)(例如,其重或輕鏈))。The invention also more particularly relates to an isolated and/or recombinant nucleic acid comprising a nucleotide sequence encoding a human immunoglobulin, a mouse immunoglobulin or a chimeric immunoglobulin, which has binding specificity for human CD52 (for example, a humanized immunoglobulin of the present invention, wherein non-human parts (for example, CDRs) are derived from mouse anti-CD52 monoclonal antibody; mouse immunoglobulin of the present invention; or chimeric immunosphere of the present invention A protein in which a non-human portion (eg, VH and VL) is derived from a mouse anti-CD52 monoclonal antibody) or a portion thereof (eg, an antigen-binding portion) (eg, a heavy or light chain thereof)).

本發明的核酸可用於製造具有對人類CD52結合專一性的人類化免疫球蛋白、有具對人類CD52結合專一性的老鼠免疫球蛋白及具有對人類CD52結合專一性的嵌合免疫球蛋白。例如,編碼本發明人類化免疫球蛋白、老鼠免疫球蛋白或嵌合免疫球蛋白的核酸(例如,DNA(例如cDNA),或RNA)或一或更多核酸可併入合適構成物(例如,重組載體),以進一步操作序列或是以製造經編碼免疫球蛋白於合適宿主細胞。The nucleic acid of the present invention can be used to produce a humanized immunoglobulin having specificity for human CD52 binding, a mouse immunoglobulin having specificity for binding to human CD52, and a chimeric immunoglobulin having specificity for binding to human CD52. For example, a nucleic acid encoding a humanized immunoglobulin, mouse immunoglobulin or chimeric immunoglobulin of the invention (eg, DNA (eg, cDNA), or RNA) or one or more nucleic acids can be incorporated into a suitable construct (eg, Recombinant vector) to further manipulate the sequence or to make a coded immunoglobulin in a suitable host cell.

亦提供一種適合用於表現具有對人類CD52結合專一性的人類化免疫球蛋白、具有對人類CD52結合專一性的老鼠免疫球蛋白或具有對人類CD52結合專一性的嵌合免疫球蛋白的構成物或載體(例如,表現載體)。多種載體為可提供的,其包含在宿主細胞維持單份或多份,或是其整合至宿主細胞的染色體。可將構成物或載體引入至合適宿主細胞,及表現本發明的人類化免疫球蛋白、老鼠免疫球蛋白或嵌合免疫球蛋白的細胞,其可於培養中製造及維持。單一載體或多重載體可用於表現具有針對人類CD52的結合專一性的人類化免疫球蛋白、老鼠免疫球蛋白或嵌合免疫球蛋白。Also provided is a composition suitable for expressing a humanized immunoglobulin having specificity for human CD52 binding, a mouse immunoglobulin having specificity for human CD52 binding, or a chimeric immunoglobulin having specificity for binding to human CD52. Or a vector (eg, a expression vector). A variety of vectors are available which comprise one or more portions in the host cell, or which are integrated into the chromosome of the host cell. The construct or vector can be introduced into a suitable host cell, and a cell expressing the humanized immunoglobulin, mouse immunoglobulin or chimeric immunoglobulin of the present invention, which can be produced and maintained in culture. A single vector or multiple vectors can be used to express a humanized immunoglobulin, mouse immunoglobulin or chimeric immunoglobulin having binding specificity for human CD52.

合適的表現載體,例如哺乳動物細胞表現載體,亦可包含數個組成,其包含,但不限於一或更多下列:複製起點;選擇性標記基因;一或更多表現控制因子,例如轉錄控制因子(例如,啟動子、增強子、終止子)、及/或一或更多轉譯信號;膜標的或分泌的信號序列或前導序列。在構成物或載體,信號胜肽序列可由構成物或載體或其他來源提供,例如,可使用免疫球蛋白的轉錄及/或轉譯信號以主導表現。Suitable expression vectors, such as mammalian cell expression vectors, may also comprise several components including, but not limited to, one or more of the following: an origin of replication; a selectable marker gene; one or more expression control factors, such as transcriptional control Factors (eg, promoters, enhancers, terminators), and/or one or more translational signals; membrane-labeled or secreted signal sequences or leader sequences. In the construct or vector, the signal peptide sequence can be provided by a construct or vector or other source, for example, transcriptional and/or translational signals of the immunoglobulin can be used to dominate expression.

一種啟動子可提供用於在合適宿主細胞的表現,啟動子可為組成型或是誘導型,例如,啟動子可操作地結合至編碼人類化免疫球蛋白或免疫球蛋白鏈的核酸,使得其主導經編碼多肽的表現。原核生物(例如,大腸桿菌的lac、tac、T3、T7啟動子)及真核生物(例如,酵母菌類醇脫氫酵素(ADH1)、SV40、CMV)宿主的各種合適啟動子為可提供的。熟知該技藝者能夠選擇適當啟動子以表現本發明抗-CD52抗體或其部份。A promoter may be provided for expression in a suitable host cell, and the promoter may be constitutive or inducible, for example, the promoter is operably linked to a nucleic acid encoding a humanized immunoglobulin or immunoglobulin chain such that Leads the performance of the encoded polypeptide. Various suitable promoters for prokaryotes (eg, the lac, tac, T3, T7 promoters of E. coli) and eukaryotes (eg, yeast alcohol dehydrogenase (ADH1), SV40, CMV) hosts are available. Those skilled in the art will be able to select an appropriate promoter to represent an anti-CD52 antibody or portion thereof of the invention.

此外,載體(例如,表現載體)典型上包含一種選擇性標記,以選擇攜帶載體的宿主細胞,及,在可複製載體的情況,為複製起點。編碼給予抗生素或抗藥性產物的基因為常見的選擇性標記且可用於原核生物(例如,β-內醯胺酶基因(抗安比西寧)、土黴素抗性基因(土黴素抗性及真核細胞(例如,新黴素(G418或建那黴素)、鳥嘌呤磷酸核糖轉移酶(黴酚酸)、安比西寧、或潮黴素抗性基因)。二氫葉酸還原酶標記基因允許在各種宿主細胞胺甲葉酸選擇,編碼宿主營養缺陷標記的基因產物的基因(例如,LEU2、URA3、HIS3)常用作酵母菌中的選擇性標記,亦包含病毒(例如,桿狀病毒)或嗜菌體載體,及能夠整合至宿主細胞基因體的載體,例如反轉錄病毒載體之使用。In addition, the vector (e.g., expression vector) typically comprises a selectable marker to select the host cell carrying the vector, and, in the case of a replicable vector, the origin of replication. Genes encoding antibiotic or drug resistance products are common selectable markers and can be used in prokaryotes (eg, beta-endoprostanase gene (anti-Anbixin), oxytetracycline resistance gene (oxytetracycline resistance and true) Nuclear cells (eg, neomycin (G418 or Jiannamycin), guanine phosphoribosyltransferase (mycophenolic acid), ampicillin, or hygromycin resistance gene). Dihydrofolate reductase marker gene allows A variety of host cell amine folate selection, genes encoding host auxotrophic marker gene products (eg, LEU2, URA3, HIS3) are commonly used as selectable markers in yeast, and also contain viruses (eg, baculovirus) or bacteriophages A vector, and a vector capable of integration into a host cell genome, such as a retroviral vector.

於是本發明亦關於一種經分離核酸分子,其編碼本發明人類化免疫球蛋白、人類化輕鏈、人類化重鏈、老鼠免疫球蛋白、老鼠免疫球蛋白輕鏈、老鼠免疫球蛋白重鏈、嵌合免疫球蛋白、嵌合輕鏈或嵌合重鏈的序列。本發明亦關於一種經分離核酸分子,其編碼免疫球蛋白的抗原-結合部分及其鏈,由本發明核酸所編碼的多肽序列係敘述於上文及下列實例。The invention therefore also relates to an isolated nucleic acid molecule encoding a humanized immunoglobulin, a humanized light chain, a humanized heavy chain, a mouse immunoglobulin, a mouse immunoglobulin light chain, a mouse immunoglobulin heavy chain, A sequence of a chimeric immunoglobulin, chimeric light chain or chimeric heavy chain. The invention also relates to an isolated nucleic acid molecule encoding an antigen-binding portion of an immunoglobulin and a strand thereof, the polypeptide sequence encoded by the nucleic acid of the invention being described above and in the following examples.

在一些具體實施例,本發明核酸及載體編碼本發明重鏈(或其抗原-結合部分)或輕鏈(或其抗原-結合部分),可使用包含重鏈-編碼核酸與輕鏈-編碼核酸的宿主細胞以製造包含重及輕鏈(或抗體的抗原-結合部分)的抗體。重鏈-編碼核酸與輕鏈-編碼核酸可放置於個別表現載體,它們亦可放置於在相同或不同表現控制的單一表現載體。參看例如,Cabilly美國專利第6,331,415號;Fang美國專利第7,662,623號。In some embodiments, the nucleic acids and vectors of the invention encode a heavy chain (or antigen-binding portion thereof) or a light chain (or antigen-binding portion thereof) thereof, and heavy chain-encoding nucleic acids and light chain-encoding nucleic acids can be used. Host cells to produce antibodies comprising heavy and light chains (or antigen-binding portions of antibodies). The heavy chain-encoding nucleic acid and the light chain-encoding nucleic acid can be placed on individual expression vectors, which can also be placed in a single expression vector that is controlled by the same or different expression. See, for example, Cabilly U.S. Patent No. 6,331,415; and Fang U.S. Patent No. 7,662,623.

具對人類CD52結合專一性的免疫球蛋製造方法Method for producing immunoglobulin with specificity for human CD52 binding

本發明另一方面係關於一種本發明抗-人類CD52抗體的製造方法,本發明抗體可例如由編碼合適宿主細胞中抗體的一或更多重組合核酸之表現製造。宿主細胞可使用任何合適方法製造,例如,可引入此處所敘述表現構成物(例如,該一或更多載體,例如,哺乳動物細胞表現載體)至合適宿主細胞,且可維持所產生細胞(例如,於培養,於動物,於植物)在適合構成物或載體表現的條件下。合適宿主細胞可為原核生物型,其包含細菌性細胞,例如大腸桿菌(例如,菌種DH5αTM(Invitrogen,Carlsbad,CA)),枯草桿菌(B. subtilis)及/或其他合適細菌;真核生物細胞,例如真菌或酵母菌細胞(例如,嗜甲醇酵母菌(Pichia pastoris)、麴菌屬(Aspergillus sp.)、釀酒酵母(Saccharomyces cerevisiae)、裂殖性酵母菌(Schizosaccharomyces pombe)、粉色麵包黴菌(Neurospora crassa)),或是其他低級真核細胞,及高級真核細胞,例如得自昆蟲者(例如,果蠅(Drosophila Schnieder) S2細胞、Sf9昆蟲細胞(WO 94/26087(O'Connor)、TN5B1-4(HIGH 5)昆蟲細胞(Invitrogen),哺乳動物(例如,COS細胞,例如COS-1(ATCC Accession No. CRL-1650)及COS-7(ATCC Accession No. CRL-1651)、CHO(例如,ATCC Accession No. CRL-9096)、CHO DG44(Urlaub,G.及Chasin,LA.,Proc. Natl. Acac. Sci. USA,77(7):4216-4220(1980))、293(ATCC Accession No. CRL-1573)、HeLa(ATCC Accession No. CCL-2)、CV1(ATCC Accession No. CCL-70)、WOP(Dailey,L.,等.,J. Virol.,54:739-749(1985))、3T3、293T(Pear,W. S.,等.,Proc. Natl. Acad. Sci. U.S.A.,90:8392-8396(1993))、NS0細胞、SP2/0細胞、HuT 78細胞及其類似細胞)),或植物(例如,煙草、lemna(duckweed)、及藻類),(參看,例如,Ausubel,F.M.等,eds. Current Protocols in Molecular Biology,Greene Publishing Associates and John Wiley & Sons Inc.(1993))。在一些具體實施例,該宿主細胞不為多細胞生物(例如,植物或動物)的一部份,例如,其為經分離宿主細胞或是為細胞培養的一部份。Another aspect of the invention pertains to a method of making an anti-human CD52 antibody of the invention, which antibody can be produced, for example, by the expression of one or more recombinant nucleic acids encoding antibodies in a suitable host cell. The host cell can be made using any suitable method, for example, the expression constructs described herein (e.g., the one or more vectors, e.g., mammalian cell expression vectors) can be introduced into a suitable host cell, and the resulting cells can be maintained (e.g., , in culture, in animals, in plants) under conditions suitable for the performance of the construct or carrier. Suitable host cells may be prokaryotic type, which comprises a bacterial cell, such as E. coli (e.g., strain DH5α TM (Invitrogen, Carlsbad, CA )), Bacillus subtilis (B. subtilis) and / or other suitable bacteria; eukaryotic Biological cells, such as fungal or yeast cells (eg, Pichia pastoris , Aspergillus sp. , Saccharomyces cerevisiae , Schizosaccharomyces pombe , pink bread mold) ( Neurospora crassa) , or other lower eukaryotic cells, and higher eukaryotic cells, such as those obtained from insects (eg, Drosophila Schnieder S2 cells, Sf9 insect cells (WO 94/26087 (O'Connor)) , TN5B1-4 (HIGH 5) insect cells (Invitrogen), mammals (eg, COS cells, such as COS-1 (ATCC Accession No. CRL-1650) and COS-7 (ATCC Accession No. CRL-1651), CHO (eg, ATCC Accession No. CRL-9096), CHO DG44 (Urlaub, G. and Chasin, LA., Proc. Natl. Acac. Sci. USA, 77(7): 4216-4220 (1980)), 293 ( ATCC Accession No. CRL-1573), HeLa (ATCC Accession No. CCL-2), CV1 (ATCC Accession) No. CCL-70), WOP (Dailey, L., et al., J. Virol., 54: 739-749 (1985)), 3T3, 293T (Pear, WS, et al., Proc. Natl. Acad. Sci USA, 90: 8392-8396 (1993)), NS0 cells, SP2/0 cells, HuT 78 cells and the like), or plants (eg, tobacco, lemna (duckweed), and algae), (see, For example, Ausubel, FM, et al, eds. Current Protocols in Molecular Biology, Greene Publishing Associates and John Wiley & Sons Inc. (1993). In some embodiments, the host cell is not a multicellular organism (eg, a plant or animal) Part of, for example, it is an isolated host cell or part of a cell culture.

本發明亦關於一種細胞,其包含本發明核酸,例如載體(例如,表現載體)。例如,編碼人類化免疫球蛋白的重及輕鏈、老鼠免疫球蛋白的重及輕鏈、或是嵌合免疫球蛋白的重及輕鏈之核酸(亦即,一或更多核酸),具有對人類CD52結合專一性的該免疫球蛋白,或包含此種核酸的構成物(亦即,一或更多構成物,例如,亦即,一或更多載體)可藉由適合於所選擇宿主細胞的方法(例如,轉殖、轉染、電穿孔法、感染)引入合適宿主細胞,且核酸序列係,或變為,操作地連接至一或更多表現控制因子(例如,於載體,於由方法於細胞中產生的構成物,整合至宿主細胞基因體),宿主細胞可維持在適合表現的條件下(例如,在誘導物、以適當鹽類補足的合適介質、生長因子、抗生素、營養補充物等的存在下),由此製造所編碼多肽。若希望,可將所編碼蛋白(例如,人類化免疫球蛋白、老鼠免疫球蛋白、嵌合免疫球蛋白)分離,例如自宿主細胞、培養介質、或乳液中分離。此方法包含在基因轉殖動物或植物(例如,菸草)的宿主細胞(例如,乳腺細胞)中的表現(參看,例如,WO 92/03918)。The invention also relates to a cell comprising a nucleic acid of the invention, such as a vector (e.g., a expression vector). For example, a heavy and light chain encoding a human immunoglobulin, a heavy and light chain of a mouse immunoglobulin, or a nucleic acid of a heavy and light chain of a chimeric immunoglobulin (ie, one or more nucleic acids), The immunoglobulin that binds to human CD52 specificity, or a construct comprising such a nucleic acid (ie, one or more constructs, eg, one or more vectors) may be adapted to the host of choice Cellular methods (eg, transfection, transfection, electroporation, infection) are introduced into a suitable host cell, and the nucleic acid sequence is, or becomes, operably linked to one or more expression control factors (eg, on a vector, The construct produced by the method in the cell is integrated into the host cell genome), and the host cell can be maintained under conditions suitable for expression (for example, in an inducer, a suitable medium supplemented with an appropriate salt, a growth factor, an antibiotic, a nutrient) In the presence of a supplement or the like, the encoded polypeptide is thus produced. If desired, the encoded protein (eg, human immunoglobulin, mouse immunoglobulin, chimeric immunoglobulin) can be isolated, for example, from a host cell, culture medium, or emulsion. This method encompasses the expression in host cells (e.g., breast cells) of a genetically transformed animal or plant (e.g., tobacco) (see, e.g., WO 92/03918).

可製造一種融合蛋白,其中免疫球蛋白(例如,人類化免疫球蛋白;免疫球蛋白鏈)係於N-端位置、C-端位置或融合蛋白內部連結至非-免疫球蛋白基團(亦即,在自然界不會存在於免疫球蛋白的基團)。例如,一些具體實施例可由插入編碼免疫球蛋白序列的核酸至合適表現載體,例如pET載體(例如,pET-15b,Novagen)、嗜菌體載體(例如,pCANTAB 5 E,Pharmacia)、或是其他載體(例如,pRIT2T蛋白A融合載體,Pharmacia)而製造。所得構成物可引入合適宿主細胞中以表現。在表現時,可藉由合適親合基質自細胞溶解產物分離或純化一些融合蛋白(參看,例如,Current Protocols in Molecular Biology(Ausubel,F.M.等,Eds.,Vol. 2,Suppl. 26,pp. 16.4.1-16.7.8(1991))。A fusion protein can be produced in which an immunoglobulin (eg, a human immunoglobulin; an immunoglobulin chain) is linked to a non-immunoglobulin group at the N-terminal position, the C-terminal position, or the fusion protein. That is, it does not exist in the immunoglobulin group in nature. For example, some embodiments may be inserted into a nucleic acid encoding an immunoglobulin sequence into a suitable expression vector, such as a pET vector (eg, pET-15b, Novagen), a phage vector (eg, pCANTAB 5 E, Pharmacia), or other The vector (for example, pRIT2T protein A fusion vector, Pharmacia) was produced. The resulting construct can be introduced into a suitable host cell for expression. In the performance, some fusion proteins can be isolated or purified from cell lysates by a suitable affinity matrix (see, for example, Current Protocols in Molecular Biology (Ausubel, FM et al, Eds., Vol. 2, Suppl. 26, pp. 16.4.1-16.7.8 (1991)).

本發明係關於一種宿主細胞,其包含編碼此處所提供免疫球蛋白(例如,本發明人類化免疫球蛋白、人類化輕鏈或人類化重鏈、老鼠免疫球蛋白、老鼠輕鏈或老鼠重鏈、嵌合免疫球蛋白、嵌合重鏈、或嵌合輕鏈)的重組核酸。本發明亦關於一種宿主細胞,其包含編碼免疫球蛋白的抗原-結合部分或其鏈的重組核酸。在一些具體實施例,該宿主細胞包含一種此處所提及本發明重組載體(例如,表現載體,哺乳動物細胞表現載體)。The present invention relates to a host cell comprising an immunoglobulin encoded herein (eg, a humanized immunoglobulin, a humanized light chain or a humanized heavy chain, a mouse immunoglobulin, a mouse light chain or a mouse heavy chain of the invention) , a recombinant nucleic acid of a chimeric immunoglobulin, a chimeric heavy chain, or a chimeric light chain). The invention also relates to a host cell comprising a recombinant nucleic acid encoding an antigen-binding portion of an immunoglobulin or a strand thereof. In some embodiments, the host cell comprises a recombinant vector of the invention (e.g., an expression vector, a mammalian cell expression vector) as referred to herein.

本發明亦關於一種本發明免疫球蛋白或免疫球蛋白多肽鏈的製備方法,在一個具體實施例,該方法包含於適合免疫球蛋白或多肽鏈表現的條件下培養此處所敘述本發明宿主細胞(例如,包含一或更多編碼免疫球蛋白或多肽鏈的經分離核酸(例如,本發明輕鏈及重鏈、僅輕鏈、或僅重鏈),例如宿主細胞可培養於基質或於懸浮液。在一些具體實施例,該方法進一步包含純化或分離免疫球蛋白或多肽鏈的方法。The invention also relates to a method for the preparation of an immunoglobulin or immunoglobulin polypeptide chain of the invention. In a specific embodiment, the method comprises culturing a host cell of the invention as described herein under conditions suitable for expression of an immunoglobulin or polypeptide chain ( For example, an isolated nucleic acid comprising one or more immunoglobulin or polypeptide chains (eg, a light chain and a heavy chain, only a light chain, or only a heavy chain of the invention), eg, a host cell can be cultured in a substrate or in suspension In some embodiments, the method further comprises a method of purifying or isolating an immunoglobulin or polypeptide chain.

本發明亦關於一種經由嗜菌體呈現法的免疫球蛋白製備方法。例如,可選別於CD52抗原上的天然抗體嗜菌體呈現庫,或者,可使用經由導向選擇的免疫球蛋白製備方法(美國專利申請案US 2006-0251658 A1.)。可產生沿例如已知抗-CD52抗體的固定重鏈(及/或輕鏈)CDR3區域建立的訂製庫,重及輕鏈的CDR1及CDR2區域可得自 天然來源(Osburn等,Methods,36:61-68(2005))。在一個具體實施例,抗-CD52 ScFvs可由ScFv nave抗體庫產生,此抗體庫係用於得到具所欲結合性質的老鼠-人類嵌合抗體。可篩選這些抗體庫以得到具所欲結合性質的抗體。可使用ScFv嗜菌體庫。例如,如在Vaughan等(1996)所敘述,辨識人類CD52的ScFvs可基本上依循一系列於重組人類CD52的重複選擇循環而從scFv導向選擇庫分離。簡言之,依循抗體庫的培養,當未經結合嗜菌體被洗掉時,預先耦合至順磁珠的免疫化抗原,及經結合嗜菌體可由磁分離回復。接著將經結合嗜菌體如在Vaughan等(1996)所敘述回復並重複選擇過程。The invention also relates to a method of preparing an immunoglobulin via a phage display method. For example, a natural antibody phage display library on the CD52 antigen may be selected, or an immunoglobulin preparation method via a guide selection may be used (US Patent Application No. US 2006-0251658 A1.). Customized libraries can be created that are established along the CDR3 region of an immobilized heavy chain (and/or light chain) such as known anti-CD52 antibodies, and the CDR1 and CDR2 regions of the heavy and light chains can be obtained from natural sources (Osburn et al, Methods, 36). :61-68 (2005)). In a specific embodiment, the anti-CD52 ScFvs can be ScFv na The ve antibody library is produced, and this antibody library is used to obtain a mouse-human chimeric antibody having the desired binding properties. These antibody libraries can be screened to obtain antibodies with the desired binding properties. A ScFv phage library can be used. For example, as described in Vaughan et al. (1996), ScFvs that recognize human CD52 can be isolated from the scFv-directed selection library essentially following a series of repeated selection cycles for recombinant human CD52. Briefly, following incubation of the antibody library, the immunogenated antigen pre-coupled to the paramagnetic beads when the unbound phage is washed away, and the bound phage can be recovered by magnetic separation. The combined phage is then reverted as described in Vaughan et al. (1996) and the selection process repeated.

在特別具體實施例,抗體庫係建構為由以單一鏈格式融合至天然人類輕鏈變異區的老鼠抗-CD52抗體的整個重鏈變異區組成。在選擇之後,辨識互補於老鼠重鏈變異區的人類輕鏈變異區,接著建構抗體庫,其為由上文所選擇人類輕鏈變異區組成,該人類輕鏈變異區以單一鏈格式融合至由天然人類CDR1及CDR2區域及得自老鼠抗-CD52抗體的重鏈變異區的固定CDR3區域所組成的嵌合重鏈變異區。在選擇CD52結合物之後,選擇最佳結合細胞株。6個CDR區域中的五個起源為人類,然而重鏈變異區的CDR-3與老鼠重鏈變異區的原先CDR3相同。In a particular embodiment, the antibody library is constructed to consist of the entire heavy chain variant region of a mouse anti-CD52 antibody fused to a native human light chain variant region in a single strand format. After selection, a human light chain variant region complementary to the mouse heavy chain variant region is identified, followed by construction of an antibody library consisting of the human light chain variant region selected above, which is fused in a single strand format to A chimeric heavy chain variant region consisting of the native human CDR1 and CDR2 regions and the fixed CDR3 region of the heavy chain variant region derived from the mouse anti-CD52 antibody. After selection of the CD52 conjugate, the optimal binding cell line was selected. Five of the six CDR regions originate from humans, whereas the CDR-3 of the heavy chain variant region is identical to the original CDR3 of the mouse heavy chain variant region.

根據製造商建議可使用耦合至Dynabeads M-270胺(Dynal)的CD52執行選擇。或者是,使用生物素化CD52的選擇可使用一級胺特定藥劑琥珀醯亞胺基-6-(生物素醯胺)己酸酯依循製造商指南製備(EZ link NHS LC Biotin,Pierce)。Selection can be performed using CD52 coupled to Dynabeads M-270 Amine (Dynal) according to the manufacturer's recommendations. Alternatively, the choice of biotinylated CD52 can be prepared using the primary amine specific agent amber imino-6-(biotin decyl) hexanoate following the manufacturer's guidelines (EZ link NHS LC Biotin, Pierce).

自選擇的輸出可基於競爭試驗於高速藥物篩選以細胞周質製備品測試,此競爭試驗測量存在於細胞周質製備品的scFvs競爭結合至CD52的能力。The self-selected output can be tested in a periplasmic preparation based on a competitive assay for high speed drug screening, which measures the ability of scFvs present in the periplasmic preparation to compete for binding to CD52.

能夠在高速藥物篩選競爭的樣品可進行DNA定序,如在Vaughan等(1996)及Osburn等(1996)所敘述。接著將選殖表現及純化為scFvs或IgGs及例如使用試驗如抗體-依賴細胞介導性細胞毒性(ADCC)試驗及補體依賴細胞毒性(CDC)試驗評估其結合CD52、中和CD52或其組合的能力。經純化scFv調製品可接著如WO 01/66754實例3所敘述製備,經純化scFv調製品的蛋白濃度可使用BCA方法(Pierce)決定。可使用類似方法以篩選固定免疫球蛋白重或輕鏈(或VH或VL)的最適配對者(相對鏈)。Samples that compete for high-speed drug screening can be subjected to DNA sequencing as described in Vaughan et al. (1996) and Osburn et al. (1996). The selection and purification are then performed as scFvs or IgGs and, for example, using assays such as antibody-dependent cell-mediated cytotoxicity (ADCC) assays and complement dependent cytotoxicity (CDC) assays to assess binding to CD52, neutralizing CD52, or a combination thereof. ability. The purified scFv preparation can then be prepared as described in Example 3 of WO 01/66754, and the protein concentration of the purified scFv preparation can be determined using the BCA method (Pierce). A similar approach can be used to screen for the most suitable pair (relative strand) of the immobilized immunoglobulin heavy or light chain (or VH or VL).

在特別具體實施例,本發明係關於一種分泌具對人類CD52的特定結合性的單株抗體的融合瘤細胞之製造方法,其包含投藥CD52基因轉殖老鼠的淋巴細胞至具有與人類CD52基因轉殖老鼠相同品系(例如,CD1)的非-基因轉殖老鼠,由此產生免疫型,非-基因轉殖老鼠。該免疫型,非-基因轉殖老鼠的脾細胞與永生細胞接觸,由此產生融合細胞,及將該融合細胞維持在製造分泌具有對人類CD52的特定結合性的單株抗體的融合瘤細胞之條件下,由此產生分泌具有對人類CD52的特定結合性的單株抗體的融合瘤細胞。In a specific embodiment, the present invention relates to a method for producing a fusion tumor cell which secretes a monoclonal antibody having specific binding to human CD52, which comprises administering a lymphocyte of a CD52 gene to a mouse to have a CD52 gene transduction with human A non-gene transgenic mouse of the same strain (eg, CD1) of the same mouse, thereby producing an immunotype, non-gene transgenic mouse. The spleen cells of the immunogenic, non-gene transgenic mouse are contacted with immortalized cells, thereby producing fused cells, and maintaining the fused cells in a fusion tumor cell which produces a monoclonal antibody having specific binding to human CD52. Under conditions, a fusion tumor cell secreting a monoclonal antibody having specific binding to human CD52 is thereby produced.

包含毒素基團或毒素的免疫球蛋白Immunoglobulin containing toxin groups or toxins

本發明亦關於一種包含毒素基團或毒素的免疫球蛋白,合適毒素基團包含毒素(例如,表面活性毒素,細胞毒素)。毒素基團或毒素可使用任何合適方法連結或共軛至免疫球蛋白。例如,毒素基團或毒素可直接或經由合適鍵合劑共價地鍵結至免疫球蛋白,合適鍵合劑可包含不可裂解或可裂解鍵合劑,例如,pH可裂解鍵合劑或包含細胞酵素(例如,細胞酯酶、細胞阮酶例如組織蛋白酶B)裂解部位的鍵合劑。此種可裂解鍵合劑可用於製備在免疫球蛋白內質化後會釋出毒素基團或毒素的免疫球蛋白。The invention also relates to an immunoglobulin comprising a toxin group or a toxin, the suitable toxin group comprising a toxin (eg, a surface active toxin, a cytotoxin). The toxin group or toxin can be linked or conjugated to the immunoglobulin using any suitable method. For example, the toxin group or toxin can be covalently bonded to the immunoglobulin, either directly or via a suitable bonding agent, and the suitable bonding agent can comprise a non-cleavable or cleavable bonding agent, for example, a pH cleavable bonding agent or comprising a cellular enzyme (eg, , a bonding agent for a cell esterase, a cell chymase such as cathepsin B) cleavage site. Such cleavable bonding agents can be used to prepare immunoglobulins that release toxin groups or toxins after endoplasmic immunoglobulins.

可使用各種方法以連結或共軛毒素基團或毒素至免疫球蛋白,所選擇特別方法依據毒素基團或毒素及所要連結或共軛的免疫球蛋白。若需要,可使用包含終端官能基的鍵合劑連結免疫球蛋白與毒素基團或毒素,一般,共軛係由將包含反應官能基(或是修飾以包含反應官能基)的毒素基團或毒素與鍵合劑或是直接與免疫球蛋白反應,共價鍵係藉由將包含(或是修飾以包含)反應基團或官能基(其在適當條件下可與第二化學基反應由此形成共價鍵)而形成。若需要,可使用任何合適方法可加入適當反應化學基至免疫球蛋白或至鍵合劑(參看,例如,Hermanson,G. T.,Bioconjugate Techniques,Academic Press: San Diego,CA(1996).)。許多合適反應化學基組合為該技藝所已知,例如胺基可與親電子基例如甲苯磺酸酯、甲磺酸酯、鹵素(氯、溴、氟、碘)、N-羥基琥珀醯亞胺酯(NHS)、及其類似物反應。硫代可與馬來醯亞胺、點乙醯基、丙烯醯、吡啶二硫物、5-硫代-2-硝基苯甲酸硫赶(TNB-硫赶)、及其類似物反應。醛官能基可耦合至含胺或含肼分子,及疊氮基可與三價磷反應以形成氨基磷酸酯或亞氨基磷酸酯鏈結。引入活化基至分子的合適方法為該技藝所已知(參看例如,Hermanson,G. T.,Bioconjugate Techniques,Academic Press: San Diego,CA(1996))。Various methods can be used to link or conjugate toxin groups or toxins to immunoglobulins, depending on the toxin group or toxin and the immunoglobulin to be linked or conjugated. If desired, a binding agent comprising a terminal functional group can be used to link the immunoglobulin to the toxin group or toxin. Typically, the conjugate is a toxin group or toxin that will contain a reactive functional group (or modified to contain a reactive functional group). Reacting with the bonding agent or directly with the immunoglobulin, the covalent bond is formed by reacting (or modifying to include) a reactive group or a functional group (which can react with the second chemical group under appropriate conditions) Formed by the price key). If desired, the appropriate reactive chemical group can be added to the immunoglobulin or to the bonding agent using any suitable method (see, for example, Hermanson, G. T., Bioconjugate Techniques, Academic Press: San Diego, CA (1996).). Many suitable reactive chemical group combinations are known in the art, such as amine groups and electrophilic groups such as tosylate, mesylate, halogen (chloro, bromo, fluoro, iodo), N-hydroxy amber imine. The ester (NHS), and its analogs react. The thio group can be reacted with maleic imine, acetophenone, propylene hydrazine, pyridine disulfide, 5-thio-2-nitrobenzoic acid sulfur (TNB-sulfur), and the like. The aldehyde functional group can be coupled to an amine-containing or ruthenium containing molecule, and the azide group can be reacted with trivalent phosphorus to form a phosphoramidate or phosphoramidate linkage. Suitable methods for introducing an activating group to a molecule are known in the art (see, for example, Hermanson, G. T., Bioconjugate Techniques, Academic Press: San Diego, CA (1996)).

合適毒素基團及毒素包含,例如,美登醇(例如,美登素醇,例如,DM1,DM4)、紫杉類、加利車黴素、倍癌黴素、或其衍生物。美登醇可為,例如,美登素醇或美登素醇類似物。美登素醇類似物的實例包含具修飾芳香環(例如,C-19-去氯基、C-20-去甲氧基、C-20-醯氧基)的類似物及具在其他位置(例如,C-9-CH、C-14-烷氧甲基、C-14-羥甲基或乙醯氧甲基、C-15-羥基/醯氧基、C-15-甲氧基、C-18-N-去甲基、4,5-去氧基)修飾的類似物。美登素醇及美登素醇類似物係敘述於美國專利第5,208,020號及第6,333,410號,其內容係併入此處做為參考。美登素醇可使用例如,N-琥珀醯亞胺3-(2-吡啶二硫基)丙酸酯(亦已知為N-琥珀醯亞胺4-(2-吡啶二硫基)戊酸酯(或SPP))、4-琥珀醯亞胺-氧羥基-a-(2-吡啶二硫基)-甲苯(SMPT)、N-琥珀醯亞胺-3-(2-吡啶二硫基)丁酸酯(SDPB)、2亞氨基硫烷、或S-乙醯基丁二酸酐而耦合至抗體或抗體片段。紫杉類可為,例如,紫杉醇、剋癌易、或新穎紫杉類(參看例如,WO 01/38318)。加利車黴素可為,例如,一種溴-複合加利車黴素(例如,α、β、或γ溴-複合),一種碘-複合加利車黴素(例如,α、β、或γ碘-複合),或是其類似物及相似物。溴-複合加利車黴素包含I1-BR、I2-BR、I3-BR、I4-BR、J1-BR、J2-BR及K1-BR,碘-複合加利車黴素包含I1-I、I2-I、I3-I、J1-I、J2-I、L1-I及K1-BR。加利車黴素及其突變物、類似物、相似物係敘述於例如美國專利第4,970,198;5,264,586;5,550,246;5,712,374、及5,714,586號,其每一個內容係併入此處做為參考。倍癌黴素類似物(例如,KW-2189、DC88、DC89 CBI-TMI、及其衍生物)係敘述於,例如,美國專利第5,070,092號、美國專利第5,187,186號、美國專利第5,641,780號、美國專利第5,641,780號、美國專利第4,923,990號、及美國專利第5,101,038號,其每一個內容係併入此處做為參考。Suitable toxin groups and toxins include, for example, maytansinol (eg, maytansinol, eg, DM1, DM4), taxanes, calicheamicin, doxorubicin, or derivatives thereof. Maytanol can be, for example, a maytansinol or maytansinol analog. Examples of maytansinol analogs include analogs with modified aromatic rings (eg, C-19-dechlorinated, C-20-desmethoxy, C-20-decyloxy) and have other positions ( For example, C-9-CH, C-14-alkoxymethyl, C-14-hydroxymethyl or ethoxymethyl, C-15-hydroxy/decyloxy, C-15-methoxy, C -18-N-desmethyl, 4,5-deoxy) modified analog. The maytansinol and maytansinol analogs are described in U.S. Patent Nos. 5,208,020 and 6,333,410, the disclosures of each of each of Maytanol can be used, for example, N-succinimide 3-(2-pyridyldithio)propionate (also known as N-succinimide 4-(2-pyridyldithio)pentanoic acid Ester (or SPP)), 4-succinimide-oxyhydroxy-a-(2-pyridyldithio)-toluene (SMPT), N-succinimide-3-(2-pyridyldithio) Butyrate (SDPB), 2 iminothiolane, or S-acetyl succinic anhydride is coupled to the antibody or antibody fragment. The taxanes can be, for example, paclitaxel, gram-free, or novel taxanes (see, for example, WO 01/38318). The calicheamicin can be, for example, a bromine-complexed calicheamicin (eg, alpha, beta, or gamma bromine-complex), an iodine-complexed calicheamicin (eg, alpha, beta, or γIodine-complex), or analogs and analogs thereof. Bromo-compound calicheamicin comprises I1-BR, I2-BR, I3-BR, I4-BR, J1-BR, J2-BR and K1-BR, and iodine-complexed calicheamicin contains I1-I, I2-I, I3-I, J1-I, J2-I, L1-I and K1-BR. The calicheamicin and its mutants, analogs, and analogs are described, for example, in U.S. Patent Nos. 4,970,198; 5,264,586; 5, 550, 246; 5, 712, 374, and 5, 714, 586, each incorporated herein by reference. The doxorubicin analogs (e.g., KW-2189, DC88, DC89 CBI-TMI, and derivatives thereof) are described in, for example, U.S. Patent No. 5,070,092, U.S. Patent No. 5,187,186, U.S. Patent No. 5,641,780, U.S. Patent No. 5, 641, 780, U.S. Patent No. 4, 923, 990, and U.S. Patent No. 5,101, 038, each of which is incorporated herein by reference.

其他毒素實例包含,但不限於抗代謝物(例如,甲氨蝶呤、6-巰嘌呤、6-巰基鳥嘌呤、阿糖胞苷、5-氟尿嘧啶decarbazine),烷化劑(例如,雙氯乙基甲胺、thioepa chlorambucil、CC-1065(參考美國專利第5,475,092、5,585,499、5,846,545號)、美法崙、卡莫司汀(BSNU)及洛莫司汀(CCNU)、環磷醯胺、白血福恩、二溴甘露糖醇、鏈佐菌素、絲裂黴素C、及順式-二氯二氨鉑(II)(DDP)順鉑)、蒽環類(例如,柔紅黴素(先前為道諾黴素)及阿霉素),抗生素(例如,更生黴素(先前為放線毒素)、博來黴素、光神黴素、絲裂黴素、嘌羅黴素安麴黴素(AMC))、倍癌黴素及其類似物或衍生物,及抗-分裂劑(例如,長春新鹼、長春花鹼、紫杉醇、auristatins(例如,auristatin E)及美登素類,及其類似物或同系物)。Examples of other toxins include, but are not limited to, antimetabolites (eg, methotrexate, 6-oxime, 6-mercaptoguanine, cytarabine, 5-fluorouracil decarbazine), alkylating agents (eg, dichloroethane) Methylamine, thioepa chlorambucil, CC-1065 (refer to U.S. Patent Nos. 5,475,092, 5,585,499, 5,846,545), melphalan, carmustine (BSNU) and lomustine (CCNU), cyclophosphamide, white blood blessing En, dibromomannitol, streptomycin, mitomycin C, and cis-dichlorodiaminoplatinum (II) (DDP) cisplatin), anthracyclines (eg, daunorubicin (previously For daunorubicin and doxorubicin), antibiotics (eg, dactinomycin (previously actinic toxin), bleomycin, mithramycin, mitomycin, puromycin ampoules ( AMC)), doxorubicin and its analogs or derivatives, and anti-splitting agents (eg, vincristine, vinblastine, paclitaxel, auristatins (eg, auristatin E) and maytansinoids, and the like Object or homologue).

毒素亦可為表面活性毒素,例如為自由基產生器(例如,含硒毒素基團),或是含放射性核素基團的毒素。合適含放射性核素基團包含例如包含放射性碘(131I或125I)、釔(90Y)、鑥(177Lu)、錒(225Ac)、鐠、砹(211At)、錸(186Re)、鉍(212Bi或213Bi)、銦(111In)、鍀(99mTc)、磷(32P)、銠(188Rh)、硫(35S)、碳(14C)、氚(3H)、鉻(51Cr)、氯(36Cl)、鈷(57Co或58Co)、鐵(59Fe)、硒(75Se)、或鎵(67Ga)的基團。The toxin may also be a surface active toxin, such as a free radical generator (eg, a selenotoxin-containing group), or a toxin containing a radionuclide group. Suitable radionuclide-containing groups include, for example, radioactive iodine (131I or 125I), hydrazine (90Y), hydrazine (177Lu), hydrazine (225Ac), hydrazine, hydrazine (211At), hydrazine (186Re), hydrazine (212Bi or 213Bi). ), indium (111In), antimony (99mTc), phosphorus (32P), antimony (188Rh), sulfur (35S), carbon (14C), antimony (3H), chromium (51Cr), chlorine (36Cl), cobalt (57Co) Or a group of 58Co), iron (59Fe), selenium (75Se), or gallium (67Ga).

毒素可為一種來自細菌來源的蛋白、多肽或肽,例如,白喉毒素、假單胞菌屬外毒素(PE)及植物蛋白(例如,蓖麻毒素A鏈(RTA)、核醣體失活蛋白(RIPs)細胞毒素、商陸抗病毒蛋白、皂草毒蛋白、及dodecandron)係意欲用作毒素。The toxin may be a protein, polypeptide or peptide derived from a bacterial source, for example, diphtheria toxin, Pseudomonas exotoxin (PE), and vegetable protein (eg, ricin A chain (RTA), ribosome inactivating protein ( RIPs) Cytotoxin, Pokeweed antiviral protein, saporin, and dodecandron are intended to be used as toxins.

設計以結合、使無法、促進負責產生特定標的蛋白的mRNA的降解或是防止其生成的核酸反義化合物亦可用作毒素。反義化合物包含反義RNA或DNA,單或雙股的,寡核甘酸,或是其類似物,其可特定地雜交至個別mRNA物種或是防止mRNA物種的轉錄及/或RNA加工及/或經編碼多肽的轉譯,及由此造成個別經編碼多肽的量的減少。Ching等Proc. Natl. Acad. Sci. U.S.A. 86: 10006-10010(1989);Broder,等,Ann. Int. Med. 113: 604-618(1990);Loreau等.,FEBS Letters 274: 53-56(1990)。有用的反義療法包含例如:Veglin TM(VasGene)及OGX-011(Oncogenix)。Nucleic acid antisense compounds designed to bind, render, inhibit, or prevent the production of mRNA responsible for the production of a particular target protein can also be used as a toxin. Antisense compounds comprise antisense RNA or DNA, single or double stranded, oligonucleotides, or analogs thereof, which specifically hybridize to individual mRNA species or prevent transcription and/or RNA processing and/or RNA processing of mRNA species and/or Translation of the encoded polypeptide, and thereby a reduction in the amount of individual encoded polypeptide. Ching et al. Proc. Natl. Acad. Sci. USA 86: 10006-10010 (1989); Broder, et al., Ann. Int. Med. 113: 604-618 (1990); Loreau et al., FEBS Letters 274: 53-56 (1990). Useful antisense therapies include, for example, VeglinTM (VasGene) and OGX-011 (Oncogenix).

毒素亦可為一種光活性劑,合適光活性劑包含樸啉-基底物質例如卟吩姆鈉、綠樸啉、二氫卟吩E6、血卟啉本身衍生物、酞花菁、etiopurpurins、替沙林、及其類似物。The toxin may also be a photoactive agent, and the suitable photoactive agent comprises a porphyrin-substrate such as sodium porphin, chlorpyrifos, chlorin E6, hematoporphyrin derivatives, phthalocyanine, etiopurpurins, and itra Forest, and its analogues.

毒素可為一種結合至细胞間標的的抗體或抗體片段,此種抗體或抗體片段可指向經定義亞細胞區間或標的,例如,抗體或抗體片段可結合至一種细胞間標的,其係由erbB2、EGFR、BCR-ABL、p21Ras、細胞凋亡蛋白酶3、細胞凋亡蛋白酶7、Bc1-2、p53、細胞週期素E、ATF-1/CREB、HPV16 E7、HP1、Type IV膠原酶、cathepsin L及其他敘述於Kontermann,R.E.,Methods,34:163-170(2004)(其係以其全文併入做為參考)的细胞間標的。The toxin may be an antibody or antibody fragment that binds to an intercellular marker, such antibody or antibody fragment may be directed to a defined subcellular interval or target, for example, an antibody or antibody fragment may be bound to an intercellular marker by erbB2. EGFR, BCR-ABL, p21Ras, apoptotic protease 3, apoptosis protease 7, Bc1-2, p53, cyclin E, ATF-1/CREB, HPV16 E7, HP1, Type IV collagenase, cathepsin L and Other inter-reports are described in Kontermann, RE, Methods, 34: 163-170 (2004), which is incorporated by reference in its entirety.

治療方法及組合物Treatment method and composition

本發明抗體有用於免疫-抑制及免疫及免疫淨化。抗體標的CD52-表現細胞(例如,T及B細胞)並減少(當用於此處時亦或"消除")於需要個體中它們的族群。淋巴細胞消耗有用於治療各種疾病及情況,例如發炎、自體免疫疾病及癌症(例如,淋巴細胞(B或T細胞)惡性腫瘤),參考例如,Reiff,A.,Hematology,10(2):79-93(2005)。可使用本發明抗體或抗原-結合部份治療的疾病及情況之實例包含但不限於多發性硬化症、狼瘡、類風濕關節炎、移植體抗宿主疾病(GVHD)、炎性腸道疾病、血管炎、貝西氏病、韋格納肉芽腫病、修格蘭氏症候群、葡萄膜炎、乾癬、硬皮症、多發性肌炎、第I型(自體免疫-基底)糖尿病、自體免疫細胞減少症(例如,自體免疫粒細胞減少症、輸血-依賴難治型PRCA、白血病及淋巴瘤例如具巨大腫瘤的非-何杰金氏淋巴瘤及B-細胞慢性淋巴性白血病。The antibodies of the invention are useful for immuno-inhibition and immune and immunopurification. The antibody-labeled CD52-expresses cells (e.g., T and B cells) and reduces (or "eliminates" when used herein) to the population in need of the individual. Lymphocyte depletion is used to treat various diseases and conditions, such as inflammation, autoimmune diseases, and cancer (eg, lymphocyte (B or T cell) malignancies), see, for example, Reiff, A., Hematology, 10(2): 79-93 (2005). Examples of diseases and conditions that may be treated using the antibodies or antigen-binding portions of the invention include, but are not limited to, multiple sclerosis, lupus, rheumatoid arthritis, graft versus host disease (GVHD), inflammatory bowel disease, blood vessels Inflammation, Beth's disease, Wegener's granulomatosis, repairing Gram's syndrome, uveitis, dryness, scleroderma, polymyositis, type I (autoimmune-basal) diabetes, autoimmune cells Reduction (eg, autoimmune neutropenia, transfusion-dependent refractory PRCA, leukemia, and lymphoma such as non-Hodgkin's lymphoma with large tumors and B-cell chronic lymphocytic leukemia).

據此,本發明方向為淋巴細胞消耗方法,及藉由投要有效量的本發明抗體至需要的個體(例如,具自體免疫疾病、血癌的人類,或是要接受移植的病人)治療發炎、自體免疫疾病及癌症的方法。亦可預防性投藥抗體至病人以預防發炎開始或是自體免疫疾病或癌症的復發,例如,本發明抗體可施藥做為a調理療法的一部分以準備病人進行移植(例如,幹細胞移植、同種異體T細胞自體移植灌注、或固體器官移植)。Accordingly, the present invention is directed to a method of lymphocyte depletion, and the treatment of inflammation by administering an effective amount of an antibody of the present invention to an individual in need thereof (for example, a human having an autoimmune disease, a blood cancer, or a patient to be transplanted). , methods of autoimmune diseases and cancer. The antibody can also be administered prophylactically to the patient to prevent the onset of inflammation or the recurrence of an autoimmune disease or cancer. For example, the antibody of the present invention can be administered as part of a conditioning therapy to prepare a patient for transplantation (eg, stem cell transplantation, homologous Autologous transplantation of allogeneic T cells, or solid organ transplantation).

本發明一些抗-CD52抗體較佳為標的某些CD52+細胞族群,一個可能解釋為這些抗體所結合的抗原決定區在CD52蛋白上包含一或更多碳水化合物基團,及此種碳水化合物基團較其他於表現一種細胞型式的CD52更為普遍,例如,我們發現抗體7F11、5F7、3G7、及11C11消耗T細胞較消耗B細胞更多,於是,這些抗抗體的人類化及嵌合抗體可用於治療T細胞惡性腫瘤且免疫抑制副作用較溫和。Some anti-CD52 antibodies of the invention are preferably a target group of certain CD52+ cells, one possibility being explained that the epitopes to which these antibodies bind comprise one or more carbohydrate groups on the CD52 protein, and such carbohydrate groups It is more common than other CD52s that express a cell type. For example, we found that antibodies 7F11, 5F7, 3G7, and 11C11 consume more T cells than B cells, so these anti-antibody humanized and chimeric antibodies can be used. Treatment of T cell malignancies with milder immunosuppressive side effects.

因為本發明抗體標的CD52-表現細胞,抗體亦可用於消耗T細胞及B細胞之外的CD52+細胞型式,例如,研究已示出血管淋巴細胞(VLC)及表現高CD52-含量的Tie2+單核細胞-骨髓樣的細胞促進腫瘤血管新生及貢獻腫瘤抗性至抗-VEGF療法。Pulaski等,J. Translational Med. 7:49(2009)。本發明抗-CD52抗體於是可藉由標的VLC及Tie2+單核細胞而用於抑制腫瘤血管新生。為此目的,抗-CD52抗體可在血管新生部位,例如腫瘤部位系統地,或局部地投藥,抗-CD52抗體療法可與照顧標準癌症治療例如化療、手術、或輻射,或是使用另一標的療法例如抗-VEGF抗體療法合併使用,抗-CD52抗體療法可用於治療,例如,乳癌、肺癌、神經膠質瘤、大腸癌、及任何其他抗-VEGF抗體的徵兆。抗-CD52抗體療法亦可用於其他血管新生情況,其包含非-腫瘤血管新生情況例如老年黃斑病變(AMD)及糖尿病視網膜病變。Because of the antibody-targeted CD52-expressing cells of the present invention, antibodies can also be used to deplete CD52+ cell types other than T cells and B cells. For example, studies have shown that vascular lymphocytes (VLC) and Tie2+ monocytes exhibit high CD52-content. - Bone marrow-like cells promote tumor angiogenesis and contribute tumor resistance to anti-VEGF therapy. Pulaski et al., J. Translational Med. 7:49 (2009). The anti-CD52 antibodies of the invention can then be used to inhibit tumor angiogenesis by the subject VLC and Tie2+ monocytes. For this purpose, anti-CD52 antibodies can be administered systemically, or locally, at angiogenic sites, such as tumor sites, and anti-CD52 antibody therapy can be used to treat standard cancer treatments such as chemotherapy, surgery, or radiation, or to use another target. Therapies such as anti-VEGF antibody therapy are used in combination, and anti-CD52 antibody therapy can be used to treat, for example, breast cancer, lung cancer, glioma, colorectal cancer, and any other anti-VEGF antibody. Anti-CD52 antibody therapy can also be used in other angiogenesis situations, including non-tumor angiogenesis conditions such as age-related macular degeneration (AMD) and diabetic retinopathy.

可單獨投藥本發明抗體至個體(例如,人類)或是在合併治療中與其他藥劑(例如,免疫抑制劑)合併投藥,抗體可在投藥額外藥劑之前,一起或之後投藥。在一些具體實施例,該額外藥劑為,例如,消炎化合物例如柳氮磺吡啶,另一種非類固醇消炎化合物,或是類固醇消炎化合物。在一些具體實施例,該額外藥劑為另一種淋巴-消耗抗體例如另一種抗-CD52抗體、抗-CD20抗體、抗-BAFF抗體、抗-BAFF-R抗體、及其類似抗體。在一些具體實施例,該額外藥劑為,例如,細胞介素、抗-細胞介素受體抗體,或可溶性受體,其扭轉、操作、及/或加強由抗-CD52抗體所媒介的淋巴消耗之後的再造過程(參看,例如,Sportes等.,「Perspective on Potential Clinical Applications of Recombinant Human Interleukin-7,」Cytokine Therapies 1182:28-38(2009))。在另一具體實施例,合成肽類似物可與本發明免疫球蛋白合併投藥。The antibody of the present invention can be administered alone to an individual (e.g., a human) or in combination therapy with other agents (e.g., an immunosuppressive agent), and the antibody can be administered together with or after administration of the additional agent. In some embodiments, the additional agent is, for example, an anti-inflammatory compound such as sulfasalazine, another non-steroidal anti-inflammatory compound, or a steroid anti-inflammatory compound. In some embodiments, the additional agent is another lymphoid-depleting antibody such as another anti-CD52 antibody, an anti-CD20 antibody, an anti-BAFF antibody, an anti-BAFF-R antibody, and the like. In some embodiments, the additional agent is, for example, an interleukin, an anti-interleukin receptor antibody, or a soluble receptor that reverses, manipulates, and/or potentiates lymphatic consumption mediated by an anti-CD52 antibody. Subsequent reengineering process (see, for example, Sportses et al., "Perspective on Potential Clinical Applications of Recombinant Human Interleukin-7," Cytokine Therapies 1182: 28-38 (2009)). In another embodiment, a synthetic peptide analog can be administered in combination with an immunoglobulin of the invention.

研究已示出藉由阿來組單抗(alemtuzumab)的淋巴細胞消耗係由嗜中性球及NK細胞所媒介(Hu等Immunology 128:260-270(2009)。於是,在合併治療的具體實施例,刺激嗜中性球及NK細胞的藥劑可在抗-CD52抗體療法之前,期間或之後投藥至病人,以增強抗體療法。刺激嗜中性球及/或NK細胞包含,但不限於(1)增加其分裂速率,(2)增加對應於抗-CD52抗體(例如,FcγRIIIa及FcγRIIIb、FcγRII、FcγRI、及FcαRI)的同種型的Fc受體的細胞表面表現,(3)移動及增加循環細胞的數目,(4)補充細胞至標的部位(例如,腫瘤、發炎、或組織損傷部位),(5)及增加其細胞毒性活性。刺激嗜中性球及/或NK細胞的藥劑實例包含,例如,粒細胞-單核細胞集落刺激因子(GM-CSF)(例如,LEUKINE或沙格司亭及莫拉司亭);粒細胞集落刺激因子(G-CSF)(例如,NEUPOGEN或非格司亭、聚乙二醇化非格司亭、及lenograstim,);CXC趨化激素受體4(CXCR4)拮抗劑(例如,MozobilTM或plerixafor);及CXC趨化激素受體2(CXCR2)拮抗劑。病人的嗜中性球數目可定期監測以確保最適治療效用,病人嗜中性球數目可在抗-CD52抗體治療開始之前測量,可基於病人的嗜中性球數目調整刺激物的數量,若病人具有較正常為低的嗜中性球數目,則可使用較高劑量的刺激物。在粒細胞減少症(其可由使用抗-CD52抗體治療而引起)期間,亦可使用較高劑量的嗜中性球刺激物以最大化抗-CD52抗體的效果。Studies have shown that lymphocyte depletion by alemtuzumab is mediated by neutrophils and NK cells (Hu et al. Immunology 128: 260-270 (2009). Thus, the specific implementation of the combination therapy For example, an agent that stimulates neutrophils and NK cells can be administered to a patient before, during or after anti-CD52 antibody therapy to enhance antibody therapy. Stimulation of neutrophils and/or NK cells includes, but is not limited to (1) Increase the rate of division, (2) increase the cell surface expression of Fc receptors corresponding to isotypes of anti-CD52 antibodies (eg, FcγRIIIa and FcγRIIIb, FcγRII, FcγRI, and FcαRI), (3) move and increase circulating cells The number, (4) supplement the cell to the target site (eg, tumor, inflammation, or tissue damage site), (5) and increase its cytotoxic activity. Examples of agents that stimulate neutrophils and/or NK cells include, for example, , granulocyte-monocyte colony-stimulating factor (GM-CSF) (eg, LEUKINE Or saxstatin and morastatin; granulocyte colony-stimulating factor (G-CSF) (eg, NEUPOGEN) Or filgrastim, pegylated filgrastim and lenograstim,); CXC chemokine receptor 4 (CXCR4) antagonists (e.g., Mozobil TM or plerixafor); and CXC chemokine receptor 2 ( CXCR2) antagonist. The patient's number of neutrophils can be monitored periodically to ensure optimal therapeutic utility. The number of neutrophils in the patient can be measured before the start of anti-CD52 antibody therapy, and the number of stimuli can be adjusted based on the number of neutrophils in the patient, if the patient Higher dose stimuli can be used with a lower number of neutrophils than normal. During neutropenia, which can be caused by treatment with an anti-CD52 antibody, higher doses of neutrophil stimuli can also be used to maximize the effect of the anti-CD52 antibody.

因為嗜中性球及/或NK細胞改善抗-CD52抗體療法的效用,合併治療的此具體實施例使得我們可對病人使用較少的抗體並維持類似的治療效果。對病人使用較少的抗體並維持治療效果可幫助減少抗-CD52抗體的副作用,其包含病人中對經投藥抗體的免疫反應及繼發性免疫(在抗-CD52抗體治療期間或之後發生的自體免疫疾病)的發展。合併治療的此具體實施例亦有用於腫瘤,例如,當病人具有粒細胞減少症。Because neutrophils and/or NK cells improve the utility of anti-CD52 antibody therapies, this particular embodiment of the combination therapy allows us to use fewer antibodies to the patient and maintain a similar therapeutic effect. The use of fewer antibodies to the patient and maintenance of the therapeutic effect may help reduce the side effects of the anti-CD52 antibody, including the immune response to the administered antibody in the patient and secondary immunization (self occurring during or after anti-CD52 antibody treatment) The development of physical immune diseases). This particular embodiment of the combination therapy is also useful for tumors, for example, when the patient has neutropenia.

在合併治療的另一具體實施例,可使用調節T細胞的刺激物以增強抗-CD52抗體療法。我們的數據顯示相較其他CD4+ T細胞,抗-CD52抗體會消耗CD4+CD25+FoxP3+調節T細胞至遠遠為低的含量,調節T細胞(亦已知為「Treg」或壓抑T細胞)為一種能夠經接觸依賴性或接觸獨立(例如,細胞介素製造)機制抑制其他淋巴細胞的增生及/或功能的細胞。已敘述數種形式的調節T細胞,其包含γδT細胞、自然殺手T(NKT)細胞、CD8+T細胞、CD4+T細胞、及雙陰性CD4-CD8-T細胞。參看,例如,Bach等,Immunol. 3:189-98(2003)。已稱CD4+CD25+FoxP3+調節T細胞為「自然發生」 調節T細胞;它們表現CD4、CD25及叉頭家族轉錄因子FoxP3(叉頭盒p3)。於是,在合併治療的此具體實施例,我們可在抗-CD52抗體治療之前、期間或之後投藥刺激CD4+CD25+FoxP3+調節T細胞的藥劑,以在淋巴細胞-消耗之後扭轉免疫系統的組成。藥劑可,例如,活化那些T細胞,穩定及/或擴充細胞族群,移動及增加細胞循環,及/或吸收細胞至標的部位。此種藥劑的實例為雷帕黴素、活性或潛伏性TGF-β(例如,TGF-β1、TGF-β2、TGF-β3、TGF-β4、及TGF-β5)、IL-10、IL-4、IFN-α、維生素D3、迪皮、及mycophenolate mofetil(參看,例如,Barrat等.,J. Exp. Med. 195:603-616(2002);Gregori等.,J Immunol. 167: 1945-1953(2001);Battaglia等,Blood 105: 4743-4748(2005);Battaglia等,J. Immunol. 177:8338-8347(2006))。In another specific embodiment of the combined therapy, stimulators that modulate T cells can be used to enhance anti-CD52 antibody therapy. Our data show that compared to other CD4+ T cells, anti-CD52 antibodies consume CD4+CD25+FoxP3+ regulatory T cells to a much lower level, regulating T cells (also known as "Treg" or suppressor T cells). A cell capable of inhibiting the proliferation and/or function of other lymphocytes via contact-dependent or contact-independent (eg, intercellular production) mechanisms. Several forms of regulatory T cells have been described which comprise γδ T cells, natural killer T (NKT) cells, CD8+ T cells, CD4+ T cells, and double negative CD4-CD8-T cells. See, for example, Bach et al, Immunol. 3:189-98 (2003). CD4+CD25+FoxP3+ regulatory T cells are known to be "naturally occurring" regulatory T cells; they display CD4, CD25 and the forkhead family transcription factor FoxP3 (fork box p3). Thus, in this specific embodiment of the combination therapy, we can administer an agent that stimulates CD4+CD25+FoxP3+ regulatory T cells before, during or after anti-CD52 antibody treatment to reverse the composition of the immune system after lymphocyte-consumption. The agent can, for example, activate those T cells, stabilize and/or expand the cell population, move and increase cell circulation, and/or absorb cells to the target site. Examples of such agents are rapamycin, active or latent TGF-β (eg, TGF-β1, TGF-β2, TGF-β3, TGF-β4, and TGF-β5), IL-10, IL-4. , IFN-α, vitamin D3, dipi, and mycophenolate mofetil (see, for example, Barrat et al., J. Exp. Med. 195: 603-616 (2002); Gregori et al., J Immunol. 167: 1945-1953 (2001); Battaglia et al, Blood 105: 4743-4748 (2005); Battaglia et al, J. Immunol. 177: 8338-8347 (2006)).

在此發明,治療一種疾病的有效量的抗-CD52抗體為一種幫助所治療個體一或更多所欲臨床終點的量例如,對狼瘡(其表現包含系統性紅斑狼瘡、狼瘡性腎炎、皮膚紅斑狼瘡、CNS狼瘡、心臟血管表現、肺表現、肝表現、血液表現、胃腸表現、肌肉骨骼表現、新生兒紅斑狼瘡、兒童全身性紅斑狼瘡、藥物誘發紅斑性狼瘡、抗磷脂症候群、及造成狼瘡表現的補體缺乏症候群;參看,例如,Robert G. Lahita,Editor,Systemic Lupus Erythematosus,4th Ed.,Elsevier Academic Press,2004),臨床終點可由監控受影響器官系統(例如,狼瘡性腎炎的血尿及/或蛋白尿)及/或使用提供數個器官系統之間疾病嚴重性的綜合分數的疾病活動性指標(例如,BILAG、SLAM、SLEDAI、ECLAM)而測量,參看,例如,Mandl等.,"Monitoring patients with systemic lupus erythematosus" in Systemic Lupus Erythematosus,4th edition,pp. 619-631,R.G. Lahita,Editor,Elsevier Academic Press,(2004)。In the present invention, an effective amount of an anti-CD52 antibody for treating a disease is an amount that helps one or more desired clinical endpoints of the treated subject, for example, for lupus (the manifestations include systemic lupus erythematosus, lupus nephritis, skin erythema Lupus, CNS lupus, cardiovascular manifestations, lung manifestations, liver manifestations, blood manifestations, gastrointestinal manifestations, musculoskeletal manifestations, neonatal lupus erythematosus, childhood systemic lupus erythematosus, drug-induced lupus erythematosus, antiphospholipid syndrome, and lupus manifestations Complement deficiency syndrome; see, for example, Robert G. Lahita, Editor, Systemic Lupus Erythematosus, 4th Ed., Elsevier Academic Press, 2004), clinical endpoints can be monitored by affected organ systems (eg, hematuria of lupus nephritis and/or Proteinuria) and/or using disease activity indicators that provide a comprehensive score of disease severity between several organ systems (eg, BILAG, SLAM, SLEDAI, ECLAM), see, for example, Mandl et al., "Monitoring patients With systemic lupus erythematosus" in Systemic Lupus Erythematosus, 4th edition, pp. 619-631, RG Lahita, Editor , Elsevier Academic Press, (2004).

在自體免疫疾病、多發性硬化症(其包含復發型、後續惡化型、初發惡化型、及惡化復發型多發性硬化症((Lublin等,Neurology 46(4),907-11(1996))的另一實例,診斷係例如在測試例如核磁共振造影(MRI)、脊髓穿刺、誘發電位檢查、及血液樣品實驗室分析協助下由徵狀歷史及神經功能檢查而進行。在MS,治療目標為減少復發的頻率及嚴重性、預防因疾病發展所產生的障礙、及促進組織修復(Compston and Coles,2008)。於是,幫助達到與該目標一致的臨床終點的抗-CD52抗體量為用於該治療的抗體的有效量。In autoimmune diseases, multiple sclerosis (which includes relapsing, subsequent worsening, initial worsening, and worsening relapsing multiple sclerosis (Lublin et al, Neurology 46(4), 907-11 (1996)) In another example, the diagnosis is performed, for example, by a test such as magnetic resonance imaging (MRI), spinal cord puncture, evoked potential examination, and laboratory analysis of blood samples, by symptom history and neurological function examination. In MS, treatment target To reduce the frequency and severity of relapses, prevent disorders due to disease progression, and promote tissue repair (Compston and Coles, 2008). Thus, the amount of anti-CD52 antibody that helps achieve clinical endpoints consistent with this goal is used An effective amount of the antibody to be treated.

為最小化致免疫性,較佳為於本發明的治療方法及組合物使用人類化抗體治療人類病患。在不需要重複投藥的情況,投藥本發明的老鼠:人類嵌合抗體至人類病患亦為合適的。To minimize immunogenicity, it is preferred to treat human patients with humanized antibodies in the methods and compositions of the invention. In the case where repeated administration is not required, administration of the mouse of the present invention: human chimeric antibody to a human patient is also suitable.

本發明的抗體可以單一單位劑量或是多重劑量在健康照顧提供者認為合適的任何時間點投藥,劑量可由該技藝已知方法決定及可依據例如個體年齡、敏感性、耐受及整體情況而定。可使用各種投藥路徑,其包含,但不限於非腸道(例如,靜脈內、動脈內、肌肉內、胞囊內、腹腔內、皮下注射)、口服(例如,飲食中)、就當時部位、局部、吸入(例如,氣管內、鼻內或口部吸入、鼻內滴劑)、或直腸,依據要治療疾病或情況而定。非腸道投藥為一種較佳投藥模式。The antibodies of the invention may be administered in a single unit dose or in multiple doses at any point deemed appropriate by the health care provider, and the dosage may be determined by methods known in the art and may depend, for example, on the age, sensitivity, tolerance, and overall condition of the individual. . A variety of routes of administration can be used, including, but not limited to, parenteral (eg, intravenous, intraarterial, intramuscular, intracystic, intraperitoneal, subcutaneous injection), oral (eg, in the diet), at the time, Topical, inhaled (eg, intratracheal, intranasal or oral inhalation, intranasal drops), or rectum, depending on the condition or condition being treated. Parenteral administration is a preferred mode of administration.

配方可依據所選擇投藥路徑而異(例如,溶液、乳液),包含要投藥抗體的適當組合物可於生理可接受媒劑或載體中製備。組合物可為多重劑量或為單一單位劑量組合物。對溶液或乳液,合適載體包含,例如,含水或醇類/水溶液、乳液或懸浮液,其包含鹽水或緩衝介質。非腸道媒劑可包含氯化鈉溶液、林格葡萄糖、葡萄糖與氯化鈉、丙醇酸酯化林格或不揮發油。靜脈內媒劑可包含各種添加劑、防腐劑、或流體、營養劑或電解質補充劑(參看,一般,Remington's Pharmaceutical Sciences,17th Edition,Mack Publishing Co.,PA,1985)。對吸入,化合物可為溶解的或是載至合適投藥用給藥器(例如,噴霧器、氣霧器或壓力噴霧器)。The formulation may vary depending on the route of administration chosen (e.g., solution, emulsion), and suitable compositions containing the antibody to be administered may be prepared in a physiologically acceptable vehicle or vehicle. The composition can be in multiple doses or in a single unit dose composition. For solutions or emulsions, suitable carriers comprise, for example, aqueous or alcoholic/aqueous solutions, emulsions or suspensions, including saline or buffering medium. Parenteral vehicles can include sodium chloride solution, Ringer's dextrose, dextrose and sodium chloride, propanolate Ringer or fixed oils. Intravenous vehicles can contain various additives, preservatives, or fluids, nutrients, or electrolyte supplements (see, generally, Remington's Pharmaceutical Sciences, 17th Edition, Mack Publishing Co., PA, 1985). For inhalation, the compound can be dissolved or loaded into a suitable pharmaceutical delivery device (eg, a nebulizer, aerosol or pressure spray).

診斷方法及組合物Diagnostic methods and compositions

本發明的免疫球蛋白亦有用於應用於研究及診斷的各種方法,例如,它們可用於偵測、分離、及/或純化人類CD52或其變化物(例如,藉由懸浮液中親合純化或是其他合適方法例如流式細胞計數法,例如,用於細胞,例如淋巴細胞),及研究人類CD52結構(例如,構形)及功能。對於活體外應用,其中抗體的致免疫性不是考量的重點,除人類化抗體之外,本發明的老鼠及嵌合抗體將為有用的。The immunoglobulins of the invention also have various methods for use in research and diagnosis, for example, they can be used to detect, isolate, and/or purify human CD52 or variants thereof (eg, by affinity purification in suspension or Other suitable methods are, for example, flow cytometry, for example, for cells, such as lymphocytes, and for studying human CD52 structures (e.g., conformation) and function. For in vitro applications where the immunogenicity of the antibody is not a critical consideration, the mouse and chimeric antibodies of the invention will be useful in addition to humanized antibodies.

本發明免疫球蛋白可用於診斷應用(例如,活體外、體外),例如,本發明人類化免疫球蛋白可用於偵測及/或量度樣品中(例如,於在組織或體液,如發炎滲出物、血液、血清、腸液、含人類CD52組織中表現人類CD52的細胞上)人類CD52的含量。樣品(例如,組織及/或體液)可得自個體及此處所敘述免疫球蛋白可用於合適免疫球蛋白方法以偵測及/或量度人類CD52表現,其包含方法例如流式細胞計數法(例如,用於懸浮液中的細胞,例如淋巴細胞),酵素連結免疫吸附法(ELISA),其包含化學發光法、放射免疫分析、及免疫組織。The immunoglobulins of the invention can be used in diagnostic applications (eg, in vitro, in vitro), for example, the humanized immunoglobulins of the invention can be used to detect and/or measure in a sample (eg, in tissue or body fluids, such as inflamed exudates) The content of human CD52 in blood, serum, intestinal fluid, cells containing human CD52 in human CD52 tissues. Samples (eg, tissue and/or body fluids) may be obtained from an individual and the immunoglobulins described herein may be used in a suitable immunoglobulin method to detect and/or measure human CD52 expression, including methods such as flow cytometry (eg, For cells in suspension, such as lymphocytes, enzyme-linked immunosorbent assay (ELISA), which includes chemiluminescence, radioimmunoassay, and immune tissue.

在一個具體實施例,提供一種偵測樣品中人類CD52的方法,其包含在合適免疫球蛋白與人類CD52的特定結合之條件下將樣品與本發明免疫球蛋白接觸並偵測所形成的抗體-CD52複合物。在應用該方法時,此處所敘述免疫球蛋白可用於分析正常比上發炎組織(例如,來自人類)的人類CD52反應性及/或表現(例如,免疫組織地),以偵測例如,炎性腸道疾病(IBD)、自體免疫疾病(例如多發性硬化及狼瘡)、癌症(例如非-何杰金氏淋巴瘤及慢性淋巴性白血病)、或其他情況與增加的人類CD52表現(例如,於受感染組織)之間的關聯。於是,本發明免疫球蛋白允許進行評估人類CD52於正常及發炎組織之存在的免疫方法,經由此可評估疾病存在、疾病進程及/或抗-人類CD52療法於疾病(例如,發炎性疾病)治療的效用。In a specific embodiment, a method of detecting human CD52 in a sample comprising contacting a sample with an immunoglobulin of the invention and detecting the formed antibody under conditions in which a suitable immunoglobulin is specifically bound to human CD52 is provided CD52 complex. In applying this method, the immunoglobulins described herein can be used to analyze human CD52 reactivity and/or performance (e.g., immunohistochemistry) in a normal inflammatory tissue (e.g., from a human) to detect, for example, inflammatory properties. Enteric disease (IBD), autoimmune diseases (such as multiple sclerosis and lupus), cancer (such as non-Hodgkin's lymphoma and chronic lymphocytic leukemia), or other conditions with increased human CD52 performance (eg, Association between infected organizations). Thus, the immunoglobulins of the present invention allow for the evaluation of immunological methods for assessing the presence of human CD52 in normal and inflamed tissues, whereby the presence of disease, disease progression and/or anti-human CD52 therapy for disease (eg, inflammatory disease) can be assessed. The utility.

此外,在以消耗抗-CD52醫療抗體的治療之後免疫球蛋白可用於檢查組織以估量該消耗多有效及以決定CD52表現是否有任何向下調節(Rawstrom等.,Br. J. Heam.,107:148-153(1999))。In addition, immunoglobulins can be used to examine tissue to assess the effectiveness of the consumption and to determine if there is any downward regulation of CD52 performance after treatment with anti-CD52 medical antibodies (Rawstrom et al., Br. J. Heam., 107). :148-153 (1999)).

除非另外定義,此處所使用所有技術及科學名稱具與熟知該技藝所普遍了解的相同意義。示例方法及物質係敘述於下文,類似或相當於此處所敘述方法及物質亦可用於本發明實務及測試。此處所提及所有出版品或其他參考文獻係以其全文併入做為參考,在衝突情況下,本專利說明書,包含定義,為優先。雖然本文引用數個文件,此引用並不構成任何這些文件形成該技藝常見一般之式的一部份之認知。在此專利說明書及申請專利範圍,要了解字眼「包含(comprise)」或變化例如「包含(comprises)」或「包含(comprising)」意味著包含所敘述整數或整數組但不排除任何其他整數或整數組。物質、方法、及實例僅為說明性及不欲為限制。Unless otherwise defined, all technical and scientific names used herein have the same meaning as commonly understood in the art. Exemplary methods and materials are described below, and methods and materials similar or equivalent to those described herein can also be used in the practice and testing of the present invention. All publications or other references mentioned herein are hereby incorporated by reference in their entirety in their entirety in the entirety in the the the the the the Although a number of documents are cited herein, this reference does not constitute an admission that any of these documents form part of the common generality of the art. In the context of this patent specification and the patent application, the words "comprise" or variations such as "comprises" or "comprising" are meant to include the recited integer or group of integers but not to exclude any other integer or Entire array. The materials, methods, and examples are illustrative only and not intended to be limiting.

示例Example 實例1:老鼠抗-人類CD52抗體的產生Example 1: Production of mouse anti-human CD52 antibody

在下列實例的老鼠抗-人類CD52抗體係由免疫化CD1品系老鼠而產生(第1A圖),所述CD1品系老鼠的脾細胞來自CD1背景的人類CD52基因轉殖老鼠,其中人類CD52於基因轉殖老鼠的老鼠B及T細胞的表面之顯示係由流式細胞計數法證實。因為基因轉殖老鼠與免疫化老鼠具有相同的背景(CD1),來自基因轉殖老鼠的脾細胞以自然格式於細胞表面呈現人類CD52為唯一、非己抗原,及免疫化非基因轉殖老鼠表現主要朝人類CD52的抗體反應。The mouse anti-human CD52 anti-system in the following examples was generated from immunized CD1 strain mice (Fig. 1A), and the spleen cells of the CD1 strain mice were derived from human CD52 gene transgenic mice with CD1 background, in which human CD52 was transgenic. The display of the surface of mouse B and T cells of the rat was confirmed by flow cytometry. Because genetically-transferred mice have the same background (ICD1) as immunized mice, spleen cells from gene-transferred mice present human CD52 as a unique, non-self antigen on the cell surface in a natural format, and immunized non-gene transgenic mice. The antibody reacts mainly to human CD52.

為收集人類CD52基因轉殖老鼠的脾細胞,將老鼠安樂死,取出脾臟並藉由通過注射器以製備單一細胞懸浮液。接著以每隻老鼠5x106的所收集人類CD52陽性脾細胞於100微升具有或不具有弗氏完全佐劑藉由腹膜內(i.p.)注射而免疫化CD1老鼠。在以每隻老鼠5x106的基因轉殖老鼠人類CD52陽性脾細胞於100微升具弗氏完全佐劑,腹膜內注射的第一次免疫化之後每兩週給予老鼠兩次追加劑量。To collect spleen cells from human CD52 gene-transferred mice, the mice were euthanized, the spleens were removed and a single cell suspension was prepared by syringe. Followed by the collection of 5x10 6 per mouse CD52-positive human spleen cells in 100 [mu] l with or without Freund's complete adjuvant by intraperitoneal (ip) injections of CD1 mice were immunized. In each rat gene transfection 5x10 6 CD52-positive human colonization of mice spleen cells with 100 microliters of complete Freund's adjuvant, the first two weeks after booster doses administered mice immunized twice intraperitoneally injected.

對於所有老鼠,在免疫化之前每隻老鼠收集其眼出血100-200微升於黃色蓋血清分離管以決定基礎位準反應性,並在第一輪免疫化之後一週決定抗-人類CD52特定免疫反應。於CHO K1細胞(設計為表現人類CD52蛋白),而不是在親代CHO K1細胞上表現高位準抗-人類CD52反應性(如由FACS測量)的老鼠,在無菌條件下收集血液及收集脾臟以產生融合瘤細胞。融合瘤細胞係在免疫化之後3-4天由使用非分泌老鼠骨髓瘤細胞系SP2/0 Ag14或NS1骨髓瘤細胞產生做為融合夥伴。將融合細胞放置於包含次黃嘌呤、胺基喋呤及胸腺嘧啶的完全生長培養基以產生融合瘤細胞。篩選後,許多融合瘤細胞上層清液,選擇許多選殖,其產生特定抗-人類CD52抗體及進一步次選殖以得到選殖族群。比例放大產生抗-人類CD52抗體的融合瘤細胞以進行進一步發展。For all mice, each mouse was collected 100-200 μl of the ocular hemorrhage in the yellow cap serum separation tube to determine the basal level reactivity before immunization, and the anti-human CD52 specific immunity was determined one week after the first round of immunization. reaction. In CHO K1 cells (designed to express human CD52 protein), rather than on high-level quasi-anti-human CD52 reactivity (as measured by FACS) on parental CHO K1 cells, blood was collected under sterile conditions and spleens were collected. Produce fusion tumor cells. The fusion tumor cell line was generated as a fusion partner by using non-secreted mouse myeloma cell line SP2/0 Ag14 or NS1 myeloma cells 3-4 days after immunization. The fused cells are placed in a complete growth medium containing hypoxanthine, aminoguanidine, and thymine to produce fusion tumor cells. After screening, a number of supernatants of the fusion tumor cells were selected for colonization, which produced specific anti-human CD52 antibodies and further colonization to obtain the selected population. Proliferation produces fusion tumor cells of anti-human CD52 antibody for further development.

實例2:老鼠抗-人類CD52抗體的重及輕鏈的PCR分析Example 2: PCR analysis of heavy and light chains of mouse anti-human CD52 antibody

數個老鼠抗-人類CD52單株抗體(第1B圖)由測試融合瘤細胞上層清液抗-人類CD52反應性的存在而辨識。選擇個別細胞株及老鼠的重及輕鏈變異序列由PCR選殖及定序辨識。與YTH 34.5 HL(亦即,Campath IG κ(大鼠)及試劑抗體CF1D12(CF1D12 κ)(Invitrogen Life Science Technologies)相較的輕鏈序列示於第2圖。類似地,與YTH 34.5 HL及試劑抗體CF1D12相較的輕鏈序列示於第3圖。Several mouse anti-human CD52 monoclonal antibodies (Panel 1B) were identified by the presence of anti-human CD52 reactivity in the supernatant of the test fusion cells. The heavy and light chain variant sequences of individual cell lines and mice were selected for PCR selection and sequencing. The light chain sequence compared to YTH 34.5 HL ( i.e., Campath IG κ (rat) and reagent antibody CF1D12 (CF1D12 κ) (Invitrogen Life Science Technologies) is shown in Figure 2. Similarly, with YTH 34.5 HL and reagents The light chain sequence compared to antibody CF1D12 is shown in Figure 3.

辨識出總共10個獨特輕鏈變異序列及11個獨特重鏈變異序列。若一個包含Campath及CF1D12,則在抗-人類CD52抗體的輕鏈內,7個獨特CDR-1區域(表1),8個獨特CDR-2區域(表2)及7個獨特CDR-3區域(表3)被辨識。A total of 10 unique light chain variant sequences and 11 unique heavy chain variant sequences were identified. If one contains Campath And CF1D12, within the light chain of the anti-human CD52 antibody, 7 unique CDR-1 regions (Table 1), 8 unique CDR-2 regions (Table 2) and 7 unique CDR-3 regions (Table 3) Recognized.

若一個包含Campath及CF1D12,則在抗-人類CD52抗體的重鏈內總共8個獨特CDR-1區域(表4),10個獨特CDR-2區域(表5)及8個獨特CDR-3區域(表6)以被辨識。If one contains Campath And CF1D12, a total of 8 unique CDR-1 regions in the heavy chain of the anti-human CD52 antibody (Table 4), 10 unique CDR-2 regions (Table 5) and 8 unique CDR-3 regions (Table 6) To be identified.

在13個不同抗-人類CD52抗體內特定輕及重鏈CDR的關連係說明於表7。The association of specific light and heavy chain CDRs within 13 different anti-human CD52 antibodies is illustrated in Table 7.

細胞株8G3.25.3.5、4G7.F3、9D9.A2、11C11.C5、3G7.E9、5F7.1.1.4、12G6.15.1.2、23E6.2.2.1、2C3.3.8.1、7F11.1.9.7及4B10.1.2.4在後文係分別稱為8G3、4G7、9D9、11C11、3G7、5F7、12G6、23E6、2C3、7F11及4B10。Cell lines 8G3.25.3.5, 4G7.F3, 9D9.A2, 11C11.C5, 3G7.E9, 5F7.1.1.4, 12G6.15.1.2, 23E6.2.2.1, 2C3.3.8.1, 7F11. 1.9.7 and 4B10.1.2.4 are referred to as 8G3, 4G7, 9D9, 11C11, 3G7, 5F7, 12G6, 23E6, 2C3, 7F11 and 4B10, respectively.

實例3:從老鼠融合瘤細胞選殖老鼠IgG變異區基因以產生老鼠/人類嵌合IgG1抗體Example 3: Selection of mouse IgG variant region genes from mouse fusion tumor cells to generate mouse/human chimeric IgG1 antibodies

主動增生及抗體分泌融合瘤細胞係用於依照製造商建議步驟流程使用Trizol試劑(Gibco/BRL)分離RNA,使用Nanodrop測量OD以定量RNA,及RNA的完整性係藉由使其在凝膠上移動或是藉由使用生物分析儀決定。總RNA反轉錄為cDNA且重及輕鏈的變異區由聚合酶連鎖反應(PCR)放大。cDNA係使用BD Sprint PowerScript反轉錄酶(Clontech)以0.5微克/微升的Oligo(dT)引子(Invitrogen Cat# Y01212)及10微莫耳濃度的反向引子(位於重及輕鏈的恆定區)(於下文以數字列出)依照製造商建議步驟流程產生。特定言之,使用編號3(SEQ ID NO: 77)、11(SEQ ID NO: 85)、19(SEQ ID NO: 93)、20(SEQ ID NO: 94)及21(SEQ ID NO: 95)的引子。使用如上文所敘述產生的cDNA執行重及輕鏈變異區的PCR放大,對重及輕鏈,皆將1微升cDNA與每一個皆10微莫耳濃度的順向引子及反向引子混合,並在2微升25毫莫耳濃度的MgCl2存在下與PCR super mix(Invitrogen)混合。PCR程序以下列步驟操作:1)95℃進行2分鐘;2)95℃進行30秒;3)56℃進行30秒;4)68℃進行45秒;5)重複步驟2至425次;6)68℃進行10分鐘及維持於16℃。於2%凝膠分析PCR產物,以偵測約300-400 bp大小的變異區序列之存在,並依照製造商指南將適當條帶選殖至pCR2.1-TOPO TA選殖套組(Invitrogen)及使用M13引子確認經選殖序列。提供用於反轉錄及用於PCR放大輕鏈及重鏈序列的引子:Active proliferation and antibody secretion fusion tumor cell lines were used to isolate RNA using Trizol reagent (Gibco/BRL) according to the manufacturer's recommended procedure, OD was quantified using Nanodrop, and RNA integrity was achieved by gel Move or decide by using a bioanalyzer. Total RNA is reverse transcribed into cDNA and the variable regions of the heavy and light chains are amplified by polymerase chain reaction (PCR). The cDNA was BD Sprint PowerScript reverse transcriptase (Clontech) with 0.5 μg/μl of Oligo (dT) primer (Invitrogen Cat# Y01212) and 10 μmol concentration of reverse primer (in the constant region of heavy and light chains) (listed below by numbers) generated in accordance with the manufacturer's recommended steps. Specifically, using numbers 3 (SEQ ID NO: 77), 11 (SEQ ID NO: 85), 19 (SEQ ID NO: 93), 20 (SEQ ID NO: 94), and 21 (SEQ ID NO: 95) The introduction. PCR amplification of the heavy and light chain variant regions was performed using the cDNA generated as described above, and for the heavy and light chains, 1 microliter of cDNA was mixed with a forward primer and a reverse primer each having a concentration of 10 micromoles. And mixed with PCR super mix (Invitrogen) in the presence of 2 microliters of 25 millimolar concentration of MgCl 2 . The PCR procedure was performed in the following steps: 1) 2 minutes at 95 °C; 2) 30 seconds at 95 °C; 3) 30 seconds at 56 °C; 4) 45 seconds at 68 °C; 5) repeated steps 2 to 425 times; It was carried out at 68 ° C for 10 minutes and at 16 ° C. The PCR product was analyzed on a 2% gel to detect the presence of a variation region sequence of approximately 300-400 bp size and the appropriate band was cloned into the pCR2.1-TOPO TA selection kit (Invitrogen) according to the manufacturer's instructions. And the selection sequence was confirmed using the M13 primer. Provide primers for reverse transcription and for PCR amplification of light and heavy chain sequences:

輕鏈引子Light chain primer

1) Lead-ML κ=5' ATGGGCWTCAARATGRARWCWCAT3'(於前導序列的順向引子)(SEQ ID NO:75)1) Lead-ML κ=5' ATGGGCWTCAARATGRARWCWCAT3' (for the forward leader of the leader sequence) (SEQ ID NO: 75)

2) FR1-ML κ=5' GAYATTGTGMTRACMCARKMTCAA 3'(於骨架1的順向引子)(SEQ ID NO:76)2) FR1-ML κ=5' GAYATTGTGMTRACMCARKMTCAA 3' (for the directional leader of backbone 1) (SEQ ID NO: 76)

3) ML κ恆定=5'ACTGGATGGTGGGAAGATGGA 3'(於恆定區的反向引子)(SEQ IDN O:77)3) ML κ constant = 5' ACTGGATGGTGGGAAGATGGA 3' (reverse primer in constant region) (SEQ ID NO: 77)

4) VK-MK=5' GAYATTGTGMTSACMCARWCTMCA 3'(於骨架1的順向引子)(SEQ ID NO:78)4) VK-MK=5' GAYATTGTGMTSACMCARWCTMCA 3' (for the forward introduction of Skeleton 1) (SEQ ID NO: 78)

5) MKC-Const=5' GGATACAGTTGGTGCAGCATC 3'(於恆定區的反向引子)(SEQ ID NO:79)5) MKC-Const=5' GGATACAGTTGGTGCAGCATC 3' (reverse primer in constant region) (SEQ ID NO: 79)

重鏈引子Heavy chain primer

6) MH-SP-ALT1=5' ATGRASTTSKGGYTMARCTKGRTT 3'(於前導序列的順向引子)(SEQ ID NO:80)6) MH-SP-ALT1=5' ATGRASTTSKGGYTMARCTKGRTT 3' (for the forward leader of the leader sequence) (SEQ ID NO: 80)

7) MH-SP-ALT2=5' ATGRAATGSASCTGGGTYWTYCTCT 3'(於前導序列的順向引子)(SEQ ID NO:81)7) MH-SP-ALT2=5' ATGRAATGSASCTGGGTYWTYCTCT 3' (for the forward leader of the leader sequence) (SEQ ID NO: 81)

8) MH-FR1=5' SAGGTSMARCTGCAGSAGTCT 3'(於骨架1的順向引子)(SEQ ID NO:82)8) MH-FR1=5' SAGGTSMARCTGCAGSAGTCT 3' (for the directional leader of backbone 1) (SEQ ID NO: 82)

9) MH-FR1-1=5' SAGGTGMAGCTCSWRSARYCSGGG 3'(於骨架1的順向引子)(SEQ ID NO:83)9) MH-FR1-1=5' SAGGTGMAGCTCSWRSARYCSGGG 3' (for the directional leader of backbone 1) (SEQ ID NO: 83)

10) MH-J2=5' TGAGGAGACTGTGAGAGTGGTGCC 3'(於J區域的反向引子)(SEQ ID NO:84)10) MH-J2=5' TGAGGAGACTGTGAGAGTGGTGCC 3' (reverse primer in the J region) (SEQ ID NO: 84)

11) MH-gamma-const=5' AYCTCCACACACAGGRRCCAGTGGATAGAC 3'(於恆定區的反向引子)(SEQ ID NO:85)11) MH-gamma-const=5' AYCTCCACACACAGGRRCCAGTGGATAGAC 3' (reverse primer in constant region) (SEQ ID NO: 85)

12) VH MH1=5' SARGTNMAGCTGSAGSAGTC 3'(於骨架1的順向引子)(SEQ ID NO:86)12) VH MH1=5' SARGTNMAGCTGSAGSAGTC 3' (for the directional primer of backbone 1) (SEQ ID NO: 86)

13) VH MH2=5' SARGTNMAGCTGSAGSAGTCWGG 3'(於骨架1的順向引子)(SEQ ID NO:87)13) VH MH2=5' SARGTNMAGCTGSAGSAGTCWGG 3' (for the forward introduction of backbone 1) (SEQ ID NO: 87)

14) VH MH3=5' CAGGTTACTCTGAAAGWGTSTG 3'(於骨架1的順向引子)(SEQ ID NO:88)14) VH MH3=5' CAGGTTACTCTGAAAGWGTSTG 3' (for the directional leader of backbone 1) (SEQ ID NO: 88)

15)VH MH4=5'GAGGTCCARCTGCAACARTC 3'(於骨架1的順向引子)(SEQ ID NO:89)15) VH MH4=5'GAGGTCCARCTGCAACARTC 3' (for the directional leader of backbone 1) (SEQ ID NO: 89)

16)VH MH5=5'CAGGTCCAACTVCAGCARCC3'(於骨架1的順向引子)(SEQ ID NO:90)16) VH MH5=5'CAGGTCCAACTVCAGCARCC3' (for the directional leader of backbone 1) (SEQ ID NO: 90)

17)VH MH6=5'GAGGTGAASSTGGTGGAATC 3'(於骨架1的順向引子)(SEQ ID NO:91)17) VH MH6=5'GAGGTGAASSTGGTGGAATC 3' (for the introversion of scaffold 1) (SEQ ID NO: 91)

18)VH MH7=5'GATGTGAACTTGGAAGTGTC 3'(於骨架1的順向引子)(SEQ ID NO:92)18) VH MH7=5'GATGTGAACTTGGAAGTGTC 3' (for the directional leader of backbone 1) (SEQ ID NO: 92)

19)IgG1=5' ATAGACAGATGGGGGTGTCGTTTTGGC 3'(於老鼠IgGl CHl恆定區的反向引子)(SEQ ID NO:93)19) IgG1 = 5' ATAGACAGATGGGGGTGTCGTTTTGGC 3' (reverse primer in mouse IgG1 CH1 constant region) (SEQ ID NO: 93)

20)IgG2A=5'CTTGACCAGGCATCCTAGAGTCA 3'(於老鼠IgG2A CHl恆定區的反向引子)(SEQ ID NO:94)20) IgG2A = 5' CTTGACCAGGCATCCTAGAGTCA 3' (reverse primer in mouse IgG2A CH1 constant region) (SEQ ID NO: 94)

21)IgG2B=5' AGGGGCCAGTGGATAGAGTGATGG 3'(於老鼠IgG2B CHl恆定區的反向引子)(SEQ ID NO:95)21) IgG2B = 5' AGGGGCCAGTGGATAGAGTGATGG 3' (reverse primer in mouse IgG2B CH1 constant region) (SEQ ID NO: 95)

退化引子導致在重鏈及輕鏈骨架1區域的5'端的一些退化。來自許多獨立重鏈變異區細胞株及來自輕鏈變異區細胞株的一致性DNA序列係用於得到胺基酸序列。Degenerate primers cause some degradation at the 5' end of the heavy and light chain backbone 1 regions. Consistent DNA sequences from a number of independent heavy chain variant region cell lines and from light chain variant region cell lines were used to obtain amino acid sequences.

功能性嵌合抗-CD52抗體係由結合重鏈及輕鏈變異區至編碼分別人類IgG1重鏈(與在Campath-1發現的序列相同)及人類κ輕鏈恆定區(與在Campath-1發現的序列相同)的DNA製造。為產生編碼CD52抗體輕鏈的pCEP4(Invitrogen)輕鏈載體,將輕鏈變異區以PCR放大及由連接酶獨立選殖至pCEP4 LIC輕鏈載體以使人類κ鏈信號序列在5'端及使輕鏈恆定區在3'端。類似地,為產生pCEP4重鏈載體,重鏈序列的變異區係由連接酶獨立選殖至pCEP4 LIC重鏈載體以使人類κ鏈信號序列在5'端及使包含CH1、樞紐區(hinge)、CH2及CH3區域的重鏈恆定區在3'端。重鏈及輕鏈的恆定區的胺基酸序列與存在於Campath1H抗體的恆定區胺基酸序列相同。The functional chimeric anti-CD52 anti-system consists of binding heavy and light chain variant regions to encode human IgG1 heavy chains, respectively (with Campath-1) The sequence found is identical) and the human kappa light chain constant region (with Campath-1) DNA found in the same sequence). To generate the pCEP4 (Invitrogen) light chain vector encoding the light chain of the CD52 antibody, the light chain variant region was amplified by PCR and independently ligated into the pCEP4 LIC light chain vector by the ligase to make the human kappa chain signal sequence at the 5' end and The light chain constant region is at the 3' end. Similarly, to generate the pCEP4 heavy chain vector, the variable region of the heavy chain sequence is independently ligated to the pCEP4 LIC heavy chain vector by the ligase to make the human kappa chain signal sequence at the 5' end and to include the CH1, hinge region (hinge) The heavy chain constant region of the CH2 and CH3 regions is at the 3' end. The amino acid sequence of the constant region of the heavy and light chains is identical to the constant region amino acid sequence present in the Campath 1H antibody.

簡言之,pCEP4 LIC載體係依照製造商建議於合適緩衝液以BfuA1(New England Biolabs-NEB)消化及在消化完成後,使用PureLink PCR純化套組(Invitrogen)純化載體。接著將線性質粒以T4DNA聚合酶(New England Biolabs)處理以產生單-股端及用於選殖變異區片段。重鏈特定pCEP4 LIC載體係用於選殖重鏈變異區及輕鏈特定pCEP4 LIC載體係用於選殖輕鏈變異區。變異區插入物係由PCR產生,其中使用包含變異區特定序列及載體懸突(overhang)的包含pCR2.1-TOPO重鏈變異區的質粒或包含pCR2.1-TOPO輕鏈變異區的質粒作為模版及引子。VENT DNA聚合酶(New England Biolabs)係用於插入物的PCR放大,以凝膠純化經PCR放大的插入物及使用T4 DNA聚合酶處理以產生單股端。將重鏈及輕鏈的經製備載體與個別變異區插入物的片段合併並於室溫培養10分鐘以用於轉殖TOPO10細胞(Invitrogen),挑選抗安比西寧細胞株及驗證其序列。將具有插入於骨架中的正確重鏈及輕鏈序列的pCEP4重鏈及pCEP4輕鏈選殖株放大及用於蛋白製造,使用陽離子脂質LipofectamineTM 2000(Invitrogen)將重鏈構築與相對應輕鏈構築以1:1的比例共轉染至HEK293細胞(Invitrogen)。轉染後三天收集經調節介質,並使用蛋白A層析純化嵌合抗體。為進行此層析方法,將介質加入蛋白A,並以50管柱體積的PBS清洗,使用5管柱體積的12.5毫莫耳濃度檸檬酸,pH 3.0沖提嵌合抗體,經沖提抗體的pH藉由加入0.5莫耳濃度HEPES中和,藉由使用PD-10凝膠過濾管柱交換使緩衝液為PBS。Briefly, the pCEP4 LIC vector was digested with BfuA1 (New England Biolabs-NEB) in a suitable buffer according to the manufacturer's recommendations and after completion of digestion, the vector was purified using PureLink PCR Purification Kit (Invitrogen). The linear plasmid was then treated with T4 DNA polymerase (New England Biolabs) to generate a single-strand end and for cloning the variant region fragments. The heavy chain specific pCEP4 LIC vector is used to select the heavy chain variant region and the light chain specific pCEP4 LIC vector for the selection of the light chain variant region. The variant region insert is generated by PCR using a plasmid comprising a pCR2.1-TOPO heavy chain variant region or a plasmid comprising a pCR2.1-TOPO light chain variant region comprising a specific region of the variant region and a vector overhang. Templates and primers. VENT DNA polymerase (New England Biolabs) is used for PCR amplification of inserts, gel purification of PCR amplified inserts and treatment with T4 DNA polymerase to produce single strands. The prepared vectors of the heavy and light chains were combined with the fragments of the individual variant inserts and incubated for 10 minutes at room temperature for transfection of TOPO10 cells (Invitrogen), anti-Ambyxin cell lines were selected and their sequences verified. Skeleton having inserted the correct heavy and light chain sequences pCEP4 heavy and light chain pCEP4 clones are amplified and used for protein manufacture using cationic lipid Lipofectamine TM 2000 (Invitrogen) heavy chain construct and a light chain corresponding to Construction was co-transfected into HEK293 cells (Invitrogen) at a ratio of 1:1. The conditioned medium was collected three days after transfection and the chimeric antibody was purified using Protein A chromatography. For this chromatographic method, the medium was added to protein A and washed with 50 column volumes of PBS, and the chimeric antibody was eluted with 5 column volumes of 12.5 millimolar citric acid, pH 3.0, and the antibody was eluted. The pH was neutralized by the addition of 0.5 molar concentration HEPES, and the buffer was PBS by using a PD-10 gel filtration column exchange.

實例4:嵌合抗-人類CD52單株抗體的抗原決定區專一性分析Example 4: Specificity analysis of epitopes of chimeric anti-human CD52 monoclonal antibodies

細胞株抗原決定區的專一性係由評估嵌合抗體結合至設計以表現由丙胺酸掃描突變誘發技術所產生的人類CD52的突變的細胞株組織能力而決定(第4圖)。CD52的12個胺基酸細胞外區域中的前10個胺基酸的抗體取代係使用STRATAGENE QUIKCHANGE II XL定點突變誘發套組於pcDNA3.1表現載體(Invitrogen)中的人類CD52 cDNA上執行。編碼野生型或突變CD52序列的pcDNA3.1載體的序列被證實,及使用LipofectamineTM轉染至CHO細胞,及藉由在包含G418的介質選擇以產生表現野生型或丙胺酸突變CD52的CHO細胞株。抗-人類CD52嵌合抗體的抗原決定區特定結合係藉由以FACS測量抗體對野生型及突變CD52表現細胞的結合而決定。FACS分析係藉由使用PE-共軛羊抗-人類二級抗體(Jackson ImmunoResearch Labs)偵測嵌合抗-CD52抗體的結合而執行。第5A-5C圖顯示抗-CD52單株抗體至野生型及突變CD52表現細胞株的平均螢光強度(MFI),即使CD52為非常短的,12個胺基酸,GPI錨定蛋白,FACS結果清楚定義有三組抗體:(1)N-端結合基團(例如4B10);(2)中間結合基團(例如4G7、9D9及11C1)與(3)C-端結合基團(例如23E6、12G6、及2C3)。抗-人類CD52單株抗體(由在實例2最後所敘述的簡寫名稱所辨識)的抗原決定區專一性係摘要於表8。The specificity of the epitope of the cell line is determined by assessing the binding of the chimeric antibody to the ability of the cell line designed to express the mutation of human CD52 produced by the alanine scanning mutation induction technique (Fig. 4). Antibody substitutions of the first 10 amino acids in the 12 amino acid extracellular regions of CD52 were performed using the STRATAGENE QUIKCHANGE II XL site-directed mutagenesis kit on human CD52 cDNA in the pcDNA3.1 expression vector (Invitrogen). CD52 encoding wild type or mutant sequence was confirmed pcDNA3.1 vector sequences, using Lipofectamine TM and transfected into CHO cells, and by selecting in G418 containing medium to produce wild-type expression of CD52 or alanine mutant CHO cell line . The epitope-specific binding of the anti-human CD52 chimeric antibody is determined by measuring the binding of the antibody to wild-type and mutant CD52-expressing cells by FACS. FACS analysis was performed by detecting binding of chimeric anti-CD52 antibodies using a PE-conjugated goat anti-human secondary antibody (Jackson ImmunoResearch Labs). Figure 5A-5C shows the mean fluorescence intensity (MFI) of anti-CD52 monoclonal antibody to wild-type and mutant CD52-expressing cell lines, even though CD52 is very short, 12 amino acids, GPI-anchored protein, FACS results Three sets of antibodies are clearly defined: (1) N-terminal binding groups (eg 4B10); (2) intermediate binding groups (eg 4G7, 9D9 and 11C1) and (3) C-terminal binding groups (eg 23E6, 12G6) And 2C3). The epitope of the anti-human CD52 monoclonal antibody (identified by the short name described at the end of Example 2) is summarized in Table 8.

CD52為一種極小的抗原但擁有相當大的,親水性N-連結醣基團及疏水性GPI-錨定。為探測糖可能構成所有或部分由抗-CD52抗體所辨識的抗原決定區之可能性,得自CHO-CD52細胞的經親合純化CD52樣品以內切醣苷酶、PNGase-F處理,以自抗原完全移除N-連結糖。接著將經處理及模擬-處理控制樣品以SDS-PAGE解析,轉漬至聚偏二氟乙烯(PVDF)薄膜(Invitrogen),以每一個3微克/毫升的抗-CD52嵌合單株抗體探測,及接著根據標準西方轉漬法步驟使用增強化學發光偵測發展,使用Campath-1H (C1H)及單獨使用(2° Alone)的轉漬係分別操作以作為陽性及陰性對照,及使用每一個單株抗體(第5D圖)探測。結果顯示抗體間對醣化比上去-醣化CD52的不同結合偏好。此特性使得將十一個抗體分類為四種形式的結合組:CD52 is a very small antigen but possesses a relatively large, hydrophilic N-linked sugar group and a hydrophobic GPI-anchoring. To detect the possibility that the sugar may constitute all or part of the epitope determined by the anti-CD52 antibody, the affinity-purified CD52 sample from CHO-CD52 cells is treated with endoglycosidase, PNGase-F, and completely from the antigen. Remove the N-linked sugar. The treated and mock-treated control samples were then analyzed by SDS-PAGE and transferred to a polyvinylidene fluoride (PVDF) film (Invitrogen) for detection of each anti-CD52 chimeric antibody at 3 μg/ml. And then using the enhanced chemiluminescence detection development according to the standard Western blotting procedure, using Campath-1H (C1H) and the individual use (2° Alone) were separately manipulated as positive and negative controls, and each monoclonal antibody (Fig. 5D) was used for detection. The results show different binding preferences for saccharification between antibodies compared to up-glycosylated CD52. This property allows eleven antibodies to be classified into four forms of binding:

1. 顯現對醣化比去-醣化CD52沒有明顯偏好之結合的抗體(4G7,9D9)1. Appearing antibodies that bind to glycosylation without depletion of glycosylated CD52 (4G7, 9D9)

2. 顯現對醣化CD52結合特定的抗體(7F11,4B10)2. Visualization of specific antibodies to glycosylated CD52 (7F11, 4B10)

3. 顯現對去-醣化CD52結合特定的抗體(8G3)3. Visualization of de-glycosylated CD52 binding to specific antibodies (8G3)

4. 顯現與醣化相較具去-醣化CD52偏好結合的抗體(12G6,5F7,23E6,2C3,11C11,3G7)4. Appearing antibodies that bind to glycosylated CD52 with de-glycosylation (12G6, 5F7, 23E6, 2C3, 11C11, 3G7)

實例5:嵌合抗-CD52抗體的CDC活性Example 5: CDC activity of chimeric anti-CD52 antibody

如下文所敘述執行補體依賴細胞毒性(CDC)檢測,簡言之,設計為表現CD52蛋白(CHO-CD52)的CHO K1細胞係用作標的細胞及以Na2 51CrO4(New England Nuclear,Boston,MA)於37℃標記1-2小時。洗滌細胞,使用X-Vivo介質再懸浮,及與抗-人類CD52抗體混合至2.2微克/毫升的最終濃度,加入人類補體(Sigma)至實驗孔以達10%的最終濃度,在1-5-小時培養之後,自每一孔收集25微升不含細胞的上層清液及以MICROBETA TRILUX閃爍計數器(Wallac,Gaithersburg,MD)計數。自發釋出的51Cr量係由單獨在介質中培養標的細胞而得到。自標的細胞的自發釋出典型上小於20%。所併入51Cr總量係由加入1% Triton X-100至蒸餾水中而決定,且裂解百分率係如下計算:[(樣品計數每分鐘(c.p.m.)-自發c.p.m.)/(總c.p.m.-自發c.p.m.)]X 100。Complement-dependent cytotoxicity (CDC) assays were performed as described below. Briefly, CHO K1 cell lines designed to express CD52 protein (CHO-CD52) were used as target cells and Na 2 51 CrO 4 (New England Nuclear, Boston) , MA) was labeled at 37 ° C for 1-2 hours. The cells were washed, resuspended in X-Vivo medium, and mixed with anti-human CD52 antibody to a final concentration of 2.2 μg/ml, and human complement (Sigma) was added to the experimental wells to a final concentration of 10% at 1-5- After hourly incubation, 25 microliters of cell free supernatant was collected from each well and counted in a MICROBETA TRILUX scintillation counter (Wallac, Gaithersburg, MD). The spontaneously released amount of 51 Cr is obtained by culturing the target cells alone in the medium. The spontaneous release of self-labeled cells is typically less than 20%. The total amount of 51 Cr incorporated was determined by the addition of 1% Triton X-100 to distilled water, and the percentage of lysis was calculated as follows: [(sample count per minute (cpm) - spontaneous cpm) / (total cpm - spontaneous cpm) ]X 100.

十二個不同的嵌合抗-CD52抗體(老鼠變異區及人類IgG1恆定區)係於具有人類補體的CHO-CD52細胞上在CDC分析中測試。Campath-1H人類化抗體係用作陽性對照,陰性對照為Campath-1H null(一種Campath-1H的非-細胞-結合最少突變-於H2迴路-重鏈CDR2區域的兩點突變(K52bD及K53D;Gilliland LK等,Journal of Immunology,162:3663-3671(1999))。結果顯示嵌合抗體能夠於CD52-表現細胞媒介CDC殺傷。一些嵌合抗體媒介強健殺傷,相當於Campath或較之為佳(第6圖)。Twelve different chimeric anti-CD52 antibodies (mouse variant and human IgGl constant region) were tested in CDC assay on CHO-CD52 cells with human complement. Campath-1H The humanized anti-system was used as a positive control and the negative control was Campath-1H. Null (a kind of Campath-1H Non-cell-binding minimal mutations - two point mutations in the H2 loop-heavy chain CDR2 region (K52bD and K53D; Gilliland LK et al, Journal of Immunology, 162: 3663-3671 (1999)). The results show that the chimeric antibody is capable of killing CD52-expressing cell-mediated CDC. Some chimeric antibody vectors are robust, equivalent to Campath Or better than (Figure 6).

實例6:嵌合抗-CD52抗體的ADCC活性Example 6: ADCC activity of chimeric anti-CD52 antibody

如下文所敘述執行抗體依賴細胞毒性(ADCC)檢測,簡言之,設計為表現CD52蛋白(CHO-CD52)的CHO K1細胞係用作標的細胞及以Na2 51CrO4(New England Nuclear,Boston,MA)於37℃標記1-2小時。洗滌細胞,使用X-Vivo介質再懸浮,及與抗-人類CD52抗體混合至1.1微克/毫升的最終濃度,人類PBMC係用作效應細胞,並以1:100標的-對-效應細胞的比例加入,在6小時隔夜培養之後,自每一孔收集25微升不含細胞的上層清液及以MICROBETA TRILUX閃爍計數器(Wallac,Gaithersburg,MD)計數。自發釋出的51Cr量係由單獨在介質中培養標的細胞而得到。自標的細胞的自發釋出典型上小於20%。所併入51Cr總量係由加入1% Triton X-100至蒸餾水中而決定,且裂解百分率係如下計算:[(樣品c.p.m.-自發c.p.m.)/(總c.p.m.-自發c.p.m.)]X 100。Antibody-dependent cytotoxicity (ADCC) assays were performed as described below, in short, CHO K1 cell lines designed to express CD52 protein (CHO-CD52) were used as target cells and Na 2 51 CrO 4 (New England Nuclear, Boston) , MA) was labeled at 37 ° C for 1-2 hours. The cells were washed, resuspended in X-Vivo medium, and mixed with anti-human CD52 antibody to a final concentration of 1.1 μg/ml. Human PBMC lines were used as effector cells and added at a ratio of 1:100-pair-effector cells. After 6 hours of overnight incubation, 25 microliters of cell free supernatant was collected from each well and counted in a MICROBETA TRILUX scintillation counter (Wallac, Gaithersburg, MD). The spontaneously released amount of 51 Cr is obtained by culturing the target cells alone in the medium. The spontaneous release of self-labeled cells is typically less than 20%. The total amount of 51 Cr incorporated was determined by the addition of 1% Triton X-100 to distilled water, and the percentage of cleavage was calculated as follows: [(sample cpm-spontaneous cpm) / (total cpm-spontaneous cpm)] X 100.

十二個不同的嵌合抗-CD52抗體(老鼠變異區及人類IgG1恆定區)係於使用人類PBMC作為效應細胞的ADCC分析中測試。Campath-1H人類化抗體係用作陽性對照,用作陰性對照的是Campath-1H null(一種Campath-1H的非-細胞-結合最少突變-於H2迴路-重鏈CDR2區域的兩點突變(K52bD及K53D;Gilliland,1999,supra)。結果顯示嵌合抗體能夠於CD52-表現細胞媒介ADCC殺傷。一些嵌合抗體媒介強健殺傷,相當於Campath-1H或較之為佳(第7圖)。Twelve different chimeric anti-CD52 antibodies (mouse variant and human IgGl constant region) were tested in ADCC assays using human PBMCs as effector cells. Campath-1H The humanized anti-system was used as a positive control and the negative control was Campath-1H. Null (a kind of Campath-1H Non-cell-binding minimal mutations - two-point mutations in the H2 loop-heavy chain CDR2 region (K52bD and K53D; Gilliland, 1999, supra ). The results show that the chimeric antibody is capable of killing in CD52-expressing cellular mediator ADCC. Some chimeric antibody media is robust, equivalent to Campath-1H Or better than it (Figure 7).

實例7:結合嵌合抗-CD52抗體至經定義淋巴細胞族群之評估Example 7: Evaluation of binding chimeric anti-CD52 antibodies to defined lymphocyte populations

使用下列螢光染劑共軛抗體於流式細胞分析:抗-CD3-FITC、抗-CD27-PE、抗-CD62L-PE Cy5、抗-CD56-PE Cy7、抗-CD16-APC Cy7(BD Biosciences,San Diego,CA)、抗-CD45RA-ECD(Beckman Coulter)、抗-CD19-太平洋藍、抗-CD4-APC Cy5.5及抗-CD8太平洋橙(Invitrogen,CA)。所有老鼠嵌合抗-人類CD52抗體及人類化Campath-1H都共軛至Alexa fluor 647(BD Pharmingen)。健康人類週邊血液單核細胞係得自冷藏保存白血球衣或是得自自商業廠商(Bioreclamation,NY,USA)所提供正常捐贈者的血液分離的單核細胞。為進行單核細胞的增長,使用磷酸生理食鹽水(PBS)以1:1稀釋人類週邊血液及小心地分層置於聚蔗糖-泛影葡胺(GE Healthcare Bio-Sciences,Uppsala,Sweden)上及於室溫離心30分鐘。取出單核細胞的中間相層及於包含5%胎牛血清(FACS緩衝液)的PBS中洗滌。汙染的紅血球細胞(RBCs)以RBC裂解溶液(Sigma,St. Louis,MO,USA)裂解,將細胞再懸浮於冷FACS緩衝液及使用40微米過濾器移除碎屑,執行十色流式細胞分析以評估9個嵌合抗-人類CD52抗體(4B10、7F11、9D9、5F7、2C3、4G7、23E6、8G3、3G7)與Campath-1H相較的結合能力。Flow cytometric analysis was performed using the following fluorescent dye conjugated antibodies: anti-CD3-FITC, anti-CD27-PE, anti-CD62L-PE Cy5, anti-CD56-PE Cy7, anti-CD16-APC Cy7 (BD Biosciences) , San Diego, CA), anti-CD45RA-ECD (Beckman Coulter), anti-CD19-Pacific blue, anti-CD4-APC Cy5.5, and anti-CD8 Pacific Orange (Invitrogen, CA). All mouse chimeric anti-human CD52 antibodies and humanized Campath-1H Both are conjugated to Alexa fluor 647 (BD Pharmingen). Healthy human peripheral blood mononuclear cell lines were obtained from cryopreserved white blood jerseys or mononuclear cells isolated from the blood of normal donors provided by commercial manufacturers (Bioreclamation, NY, USA). For monocyte growth, human peripheral blood was diluted 1:1 with phosphoric acid saline (PBS) and carefully layered onto Ficoll-Hypasamine (GE Healthcare Bio-Sciences, Uppsala, Sweden) And centrifuge at room temperature for 30 minutes. The mesophase layer of monocytes was removed and washed in PBS containing 5% fetal bovine serum (FACS buffer). Contaminated red blood cells (RBCs) were lysed with RBC lysis solution (Sigma, St. Louis, MO, USA), resuspended in cold FACS buffer and debris removed using a 40 micron filter to perform ten-color flow cytometry Analysis to evaluate 9 chimeric anti-human CD52 antibodies (4B10, 7F11, 9D9, 5F7, 2C3, 4G7, 23E6, 8G3, 3G7) with Campath-1H Compared to the ability to combine.

簡言之,1 x 106 PBMC's於FACS緩衝液的重複物使用對CD3、CD27、CD45RA、CD62L、CD56、CD19、CD8、CD4、CD16的抗體與9個嵌合抗-人類CD52抗體(4B10、7F11、9D9、5F7、2C3、4G7、23E6、8G3、3G7)其中一個的預先-滴定稀釋液之混合物於4℃培養30分鐘。洗滌細胞及固定於包含1%多聚甲醛的PBS。100,000個染色細胞於BD LSR-II(BD Biosciences,San Jose,CA)上得到,及使用FlowJo 7.2版軟體(Tree Star,Inc,Oregan,USA)分析數據。具不同表現型特徵的多個子集已在B及T淋巴細胞之間定義且已顯示CD52要表現於所有人類淋巴細胞。執行十色流式細胞分析以辨識淋巴細胞子集,及以評估抗-CD52抗體與在所定義子集上細胞表面CD52的結合特徵之相似點及不同點。使用標記組合,對應於B、T及NK細胞系的11個表現型不同細胞族群先自淋巴球路徑(lymphocyte gate)定義出。接著評估對應於抗-CD52抗體偵測CD52表現的能力之染色強度。統計表(第8A-8C圖)顯示個別淋巴細胞族群上以每一個抗體偵測CD52的程度之比較。數據顯示抗體在結合至CD52方面展現顯著不同。4B10、9D9、7F11及Campath-1H的偵測程度為可相較的,於幾乎所有檢查的細胞子集,雖然4B10一致地顯示較包含Campath-1H的其他抗體為最高的偵測程度。另一方面,使用3G7、4G7、8G3及23E6抗體的CD52偵測程度顯著為低。結果顯示在抗體之間相關於辨識不同細胞族群上CD52的能力之層次,4B10為最高及3G7為最低。令人有興趣地是,於CD4效應細胞,這些差別較不明顯,及在NK細胞子集較明顯,於此CD52顯示出在相當較低位準表現。在結合特徵的差異顯示嵌合抗體的性質不僅與Campath-1H顯著不同,亦反應在抗體之間性質的差別。Briefly, 1 x 10 6 PBMC's in FACS buffer replicates antibodies against CD3, CD27, CD45RA, CD62L, CD56, CD19, CD8, CD4, CD16 and 9 chimeric anti-human CD52 antibodies (4B10, A mixture of pre-titration dilutions of one of 7F11, 9D9, 5F7, 2C3, 4G7, 23E6, 8G3, 3G7) was incubated at 4 ° C for 30 minutes. The cells were washed and fixed in PBS containing 1% paraformaldehyde. 100,000 stained cells were obtained on BD LSR-II (BD Biosciences, San Jose, CA) and data were analyzed using FlowJo version 7.2 software (Tree Star, Inc, Oregan, USA). Multiple subsets with different phenotypic characteristics have been defined between B and T lymphocytes and it has been shown that CD52 is to be expressed in all human lymphocytes. A ten-color flow cytometric analysis was performed to identify subsets of lymphocytes and to assess similarities and differences in the binding characteristics of anti-CD52 antibodies to cell surface CD52 on defined subsets. Using a combination of markers, 11 phenotype-specific cell populations corresponding to the B, T, and NK cell lines were first defined from the lymphocyte gate. The staining intensity corresponding to the ability of the anti-CD52 antibody to detect CD52 expression was then evaluated. The statistical table (Fig. 8A-8C) shows a comparison of the extent to which CD52 is detected by each antibody on individual lymphocyte populations. The data shows that antibodies exhibit significant differences in binding to CD52. 4B10, 9D9, 7F11 and Campath-1H The degree of detection is comparable to that of almost all examined cell subsets, although 4B10 consistently shows more than Campath-1H Other antibodies are the highest level of detection. On the other hand, the degree of CD52 detection using the 3G7, 4G7, 8G3 and 23E6 antibodies was significantly low. The results show a level of correlation between antibodies in identifying CD52 on different cell populations, with 4B10 being the highest and 3G7 being the lowest. Interestingly, these differences were less pronounced in CD4 effector cells and were more pronounced in the NK cell subset, where CD52 showed a relatively low level of performance. Differences in binding characteristics show the properties of chimeric antibodies not only with Campath-1H Significantly different, it also reflects the difference in properties between antibodies.

實例8:人類CD52基因轉殖老鼠中嵌合抗-CD52抗體之分析(7F11、8G3、23E6、12G6、4B10及5F7)Example 8: Analysis of chimeric anti-CD52 antibodies in human CD52 transgenic mice (7F11, 8G3, 23E6, 12G6, 4B10 and 5F7)

或嵌合抗-CD52抗體(7F11、8G3、23E6、12G6、4B10及5F7)投藥至人類CD52基因轉殖老鼠,以檢查淋巴細胞消耗的程度。將100微升體積的Campath或嵌合抗-CD52抗體以1毫克/公斤的劑量腹膜內注射至老鼠。三天之後殺死老鼠並收集血液及脾臟以決定B及T-細胞消耗的位準。利用流式細胞計數法評估存在於huCD52基因轉殖老鼠的循環週邊血液或脾臟的總T輔助細胞、細胞毒性T細胞、及B細胞之絕對數。這些淋巴細胞族群係由其下列蛋白抗原的表面表現而定義:CD4表現辨識T輔助細胞族群,CD8表現辨識細胞毒性T細胞族群及CD19表現辨識所有成熟B細胞族群。顯著位準的T及B-細胞消耗於12G6及4B10抗體皆可觀察到,其可與使用所觀察到的消耗相較。使用、嵌合12G6或嵌合4B10抗體的處理顯著降低在此劑量位準經處理老鼠的血液及脾臟中的T及B細胞,7F11及5F7嵌合抗體造成血液及脾臟中顯著位準的T細胞消耗位準但是在消耗血液及脾臟中B細胞為較不有效的。以23E6抗體處理產生在此劑量的中等位準的消耗,然而使用較低親合8G3抗體會觀察到些微甚至沒有消耗。Take Or chimeric anti-CD52 antibodies (7F11, 8G3, 23E6, 12G6, 4B10 and 5F7) were administered to human CD52 gene-transferred mice to examine the extent of lymphocyte depletion. Will be 100 microliters of Campath Or chimeric anti-CD52 antibody was injected intraperitoneally into mice at a dose of 1 mg/kg. After three days, the mice were killed and blood and spleen were collected to determine the level of B and T-cell consumption. The absolute number of total T helper cells, cytotoxic T cells, and B cells present in circulating peripheral blood or spleen of huCD52 gene-transferred mice was evaluated by flow cytometry. These lymphocyte populations are defined by the surface manifestations of the following protein antigens: CD4 expression identifies T helper cell populations, CD8 expression identifies cytotoxic T cell populations, and CD19 expression recognizes all mature B cell populations. Significant levels of T and B-cell consumption can be observed in both 12G6 and 4B10 antibodies, which can be used with The observed consumption is comparable. use Treatment with chimeric 12G6 or chimeric 4B10 antibody significantly reduced T and B cells in the blood and spleen of this dose-treated mice, and 7F11 and 5F7 chimeric antibodies caused significant levels of T-cell depletion in blood and spleen. Level but B cells are less effective in consuming blood and spleen. Treatment with the 23E6 antibody produced a moderate level of consumption at this dose, however little or no consumption was observed with the lower affinity 8G3 antibody.

第9A-9C圖顯示在使用嵌合抗體給藥之後72小時的血液中CD4T細胞、CD8T細胞及CD19B細胞的含量。第10A-10C圖顯示在給藥之後72小時脾臟中CD4T細胞、CD8T細胞及CD19B細胞的含量。Figures 9A-9C show the levels of CD4 T cells, CD8 T cells and CD19B cells in the blood 72 hours after administration with the chimeric antibody. Figures 10A-10C show the levels of CD4 T cells, CD8 T cells and CD19 B cells in the spleen 72 hours after dosing.

實例9:人類CD52基因轉殖老鼠中嵌合抗-CD52抗體之分析(2C3、3G7、4B10、9D9、及11C11)Example 9: Analysis of chimeric anti-CD52 antibodies in human CD52 transgenic mice (2C3, 3G7, 4B10, 9D9, and 11C11)

或嵌合抗-CD52抗體(2C3、3G7、4B10、9D9及11C11)投藥至人類CD52基因轉殖老鼠以檢查淋巴細胞消耗的程度。將100微升體積的Campath或嵌合抗-CD52抗體以1毫克/公斤的劑量腹膜內注射至老鼠。三天之後殺死老鼠及收集血液及脾臟以決定B及T-細胞消耗的位準。利用流式細胞計數法評估存在於huCD52基因轉殖老鼠的循環週邊血液的總T輔助細胞、細胞毒性T細胞、及B細胞之絕對數。這些淋巴細胞族群係由其下列蛋白抗原的表面表現而定義:CD4表現辨識T輔助細胞族群,CD8表現辨識細胞毒性T細胞族群及CD19表現辨識所有成熟B細胞族群。顯著位準的T及B-細胞消耗於血液及脾臟抗體皆觀察到,2C3及9D9的消耗活性可與使用Campath所觀察到的消耗為相較的且顯著位準的CD4及CD8T細胞及CD19 B細胞被消耗。使用嵌合4B10的處理亦產生基因轉殖老鼠中淋巴細胞數目的顯著降低,然而使用嵌合抗體3G7或11C11抗體的處理顯著消耗血液中T細胞,所存在B細胞的位準於此劑量並未受顯著影響。will Or chimeric anti-CD52 antibodies (2C3, 3G7, 4B10, 9D9 and 11C11) were administered to human CD52 gene transgenic mice to examine the extent of lymphocyte depletion. Will be 100 microliters of Campath Or chimeric anti-CD52 antibody was injected intraperitoneally into mice at a dose of 1 mg/kg. After three days, the mice were killed and blood and spleen were collected to determine the level of B and T-cell consumption. The absolute number of total T helper cells, cytotoxic T cells, and B cells present in the circulating peripheral blood of huCD52 gene-transferred mice was evaluated by flow cytometry. These lymphocyte populations are defined by the surface manifestations of the following protein antigens: CD4 expression identifies T helper cell populations, CD8 expression identifies cytotoxic T cell populations, and CD19 expression recognizes all mature B cell populations. Significant levels of T and B-cell consumption in blood and spleen antibodies were observed, 2C3 and 9D9 depletion activity can be used with Campath The observed consumption was comparable and significant levels of CD4 and CD8 T cells and CD19 B cells were consumed. Treatment with chimeric 4B10 also produced a significant decrease in the number of lymphocytes in the transgenic mice, whereas treatment with the chimeric antibody 3G7 or 11C11 antibody significantly depleted T cells in the blood, and the presence of B cells was not at this dose. Significantly affected.

第11A-11C圖顯示在給藥嵌合抗體之後72小時血液中CD4 T細胞、CD8 T細胞及CD19 B細胞的含量。Figures 11A-11C show the levels of CD4 T cells, CD8 T cells, and CD19 B cells in the blood 72 hours after administration of the chimeric antibody.

實例10:抗-CD52抗體效用之分析(7F11、4B10及12G6)Example 10: Analysis of the utility of anti-CD52 antibodies (7F11, 4B10 and 12G6)

將100微升體積的1x106 B104腫瘤細胞注射至四十隻SCID老鼠(每組n=8)的右側腹。腫瘤細胞注射後第11天,開始使用Campath、7F11、4B10或12G6嵌合抗體處理。將抗體在剩餘實驗全程以10毫克/公斤每週一次腹膜內注射投藥,在未經處理組的所有老鼠腫瘤持續成長,在29天的中間存活期後死掉,較未經處理組,Campath的處理造成統計上顯著增加的存活(中間存活期(MS)50天及p<0.0001),嵌合抗-CD52抗體的處理亦較未經處理老鼠產生統計上顯著增加的存活(7F11與4B10的p<0.0001及12G6的p=0.0020)。基於存活率,7F11與4B10抗體的活性顯然皆較Campath為大(7F11的63%存活率及4B10的75%存活率相較於Campath的50%存活率)。第12圖顯示處理後老鼠的存活百分率。A 100 microliter volume of 1x106 B104 tumor cells was injected into the right abdomen of forty SCID mice (n=8 per group). On the 11th day after tumor cell injection, start using Campath , 7F11, 4B10 or 12G6 chimeric antibody treatment. The antibody was administered intraperitoneally at 10 mg/kg once a week for the remainder of the experiment. Tumors of all mice in the untreated group continued to grow and died after an intermediate survival period of 29 days, compared with the untreated group, Campath. Treatment resulted in a statistically significant increase in survival (intermediate survival (MS) 50 days and p < 0.0001), and chimeric anti-CD52 antibody treatment also produced statistically significantly increased survival compared to untreated mice (7F11 and 4B10). p < 0.0001 and p = 0.0020 of 12G6). Based on survival, the activity of 7F11 and 4B10 antibodies is clearly higher than that of Campath. Large (63% survival rate of 7F11 and 75% survival rate of 4B10 compared to Campath 50% survival rate). Figure 12 shows the percent survival of mice after treatment.

實例11:抗-CD52抗體效用之分析(2C3、8G3以及23E6)Example 11: Analysis of the utility of anti-CD52 antibodies (2C3, 8G3, and 23E6)

將100微升體積的1x106 B104腫瘤細胞注射至四十隻SCID老鼠(每組n=8)的右側腹。腫瘤細胞在注射後第11天,開始以Campath、2C3、8G3或23E6嵌合抗體處理。將抗體在剩餘實驗全程以10毫克/公斤每週一次腹膜內注射投藥,在未經處理組的所有老鼠的腫瘤持續成長,在26天的中間存活期後死掉,以Campath、23E6、及2C3抗體的處理產生統計上顯著增加的存活(分別為p=0.0025、p=0.0007、及p=0.0002)。第13圖顯示處理後老鼠的存活百分率。A 100 microliter volume of 1x106 B104 tumor cells was injected into the right abdomen of forty SCID mice (n=8 per group). Tumor cells start on Campo 11th day after injection , 2C3, 8G3 or 23E6 chimeric antibody treatment. The antibody was administered intraperitoneally at a dose of 10 mg/kg once a week for the remainder of the experiment. The tumors of all the mice in the untreated group continued to grow and died after an intermediate survival period of 26 days to Campath. Treatment with 23E6, and 2C3 antibodies produced statistically significant increases in survival (p=0.0025, p=0.0007, and p=0.0002, respectively). Figure 13 shows the percent survival of mice after treatment.

實例12:異種移植腫瘤模型中嵌合抗-CD52抗體效用之分析(9D9及4B10)Example 12: Analysis of the utility of chimeric anti-CD52 antibodies in xenograft tumor models (9D9 and 4B10)

將100微升體積的1x106 B104腫瘤細胞注射至四十隻SCID老鼠(每組n=8)的右側腹。腫瘤細胞在注射後第11天,開始以Campath、9D9或4B10嵌合抗體處理。將抗體在剩餘實驗全程以10毫克/公斤每週一次腹膜內注射投藥,在未經處理組的所有老鼠的腫瘤持續成長,在27天的中間存活期後死掉。以Campath的處理產生較未經處理組統計上顯著增加的存活(中間存活期未達到及p<0.0001),以嵌合抗-CD52抗體處理亦產生較未經處理老鼠統計上顯著增加的存活(9D9及4B10的p<0.0001)。存活曲線的統計分析透露在此實驗中9D9嵌合抗體顯示可與Campath相較的活性(p=0.0675)。第14圖顯示處理後老鼠的存活百分率。A 100 microliter volume of 1x106 B104 tumor cells was injected into the right abdomen of forty SCID mice (n=8 per group). Tumor cells start on Campo 11th day after injection , 9D9 or 4B10 chimeric antibody treatment. The antibody was administered intraperitoneally at a weekly dose of 10 mg/kg throughout the remainder of the experiment, and the tumors of all the mice in the untreated group continued to grow and died after an intermediate survival period of 27 days. Campath Treatment resulted in a statistically significant increase in survival compared to the untreated group (intermediate survival did not reach and p < 0.0001), and treatment with chimeric anti-CD52 antibody also produced a statistically significant increase in survival compared to untreated mice (9D9 and p<0.0001 of 4B10). Statistical analysis of survival curves revealed that 9D9 chimeric antibodies were shown to be compatible with Campath in this experiment. Relative activity (p=0.0675). Figure 14 shows the percent survival of mice after treatment.

實例13:異種移植腫瘤模型中嵌合抗-CD52抗體效用之分析(2C3及11C11)Example 13: Analysis of the utility of chimeric anti-CD52 antibodies in xenograft tumor models (2C3 and 11C11)

將100微升體積的1x106 B104腫瘤細胞注射至四十隻SCID老鼠(每組n=8)的右側腹。注射後第11天,開始以Campath、2C3或11C11嵌合抗體處理腫瘤細胞。將抗體在剩餘實驗全程以10毫克/公斤每週一次腹膜內注射投藥,在未經處理組的所有老鼠的腫瘤持續成長,在32天的中間存活期後死掉,以Campath的處理產生較未經處理組統計上顯著增加的存活(中間存活期未達到及p<0.0001),以嵌合抗-CD52抗體的處理亦產生較未經處理老鼠統計上顯著增加的存活(2C3的p<0.0001及11C11的p=0.0004)。存活曲線的統計分析透露2C3及11C11嵌合抗體顯示可與Campath相較的活性(2C3的p=0.3173及11C11的p=0.9703)。第15圖顯示使用Campath、2C3嵌合抗體或11C11嵌合抗體處理後老鼠的存活百分率。A 100 microliter volume of 1x106 B104 tumor cells was injected into the right abdomen of forty SCID mice (n=8 per group). On the 11th day after the injection, start with Campath , 2C3 or 11C11 chimeric antibodies treat tumor cells. The antibody was administered intraperitoneally at a dose of 10 mg/kg once a week for the remainder of the experiment. The tumors of all the mice in the untreated group continued to grow and died after 32 days of intermediate survival to Campath. Treatment resulted in a statistically significant increase in survival compared to the untreated group (intermediate survival did not reach and p < 0.0001), and treatment with chimeric anti-CD52 antibody also produced a statistically significant increase in survival compared to untreated mice (2C3) p<0.0001 and p=0.0004 of 11C11). Statistical analysis of survival curves revealed that 2C3 and 11C11 chimeric antibodies were shown to be compatible with Campath The activity was compared (p=0.3173 for 2C3 and p=0.9703 for 11C11). Figure 15 shows the use of Campath Percentage of survival of mice treated with 2C3 chimeric antibody or 11C11 chimeric antibody.

實例14:人類化抗-CD52抗體4B10的生成及分析Example 14: Generation and analysis of humanized anti-CD52 antibody 4B10

人類化抗人類-CD52抗體4B10係由移植老鼠4B10抗體的CDR區域至人類抗體變異區骨架而產生。老鼠4B10重鏈及輕鏈序列係由基於網路的序列排列評估以辨識用作CDR移植合適受體的人類細胞株重鏈及輕鏈骨架序列(第16圖)。由Kabat及IMGT定義CDR區域的殘基係疊合至具高序列相似度的人類骨架區域,以產生人類化重鏈及輕鏈序列,執行經疊合4B10重鏈及輕鏈序列的目視檢查及序列分析以辨識最合適的受體序列。在所有具高相似性的細胞株序列中,重鏈的VH3-72細胞株序列及輕鏈的VK2-A18b(人類細胞株序列可於Tomlinson,IM,等,EMBO J.,14(18):4628-4638(1995);Cook,GP.,等Nature Genetics,7:162-168(1994)出版品中敘述的網站發現)係因其與老鼠骨架區域有高度同源性及序列相似度,及做為CDR受體序列的最少CDR迴路結構分裂而被選擇。4B10重鏈及輕鏈的CDR1、2、及3序列係分別移植至VH3-72及VK2-A18b人類骨架區域4B10以產生人類化重鏈及輕鏈序列(說明於第17圖;第110圖)。The humanized anti-human-CD52 antibody 4B10 was produced from the CDR region of the transplanted mouse 4B10 antibody to the human antibody variant region backbone. The mouse 4B10 heavy and light chain sequences were evaluated by network-based sequence alignment to identify human cell strain heavy and light chain backbone sequences that serve as suitable receptors for CDR grafting (Fig. 16). By Kabat and IMGT Residues defining CDR regions are superimposed into human framework regions with high sequence similarity to generate humanized heavy and light chain sequences, and visual inspection and sequence analysis of overlapping 4B10 heavy and light chain sequences are performed to identify The most suitable receptor sequence. In all sequences with high similarity, the heavy chain VH3-72 cell line sequence and the light chain VK2-A18b (human cell line sequence can be found in Tomlinson, IM, et al, EMBO J., 14 (18): 4628-4638 (1995); Cook, GP., et al., Nature Genetics, 7: 162-168 (1994) published in the publication of the website) because of its high homology and sequence similarity with the mouse framework region, and Selected as the minimal CDR loop structure splitting of the CDR receptor sequences. The CDR1, 2, and 3 sequences of the 4B10 heavy and light chains were grafted to the VH3-72 and VK2-A18b human framework regions 4B10, respectively, to generate humanized heavy and light chain sequences (described in Figure 17; Figure 110). .

實例15:嵌合及人類化4B10單株抗體結合活性之評估Example 15: Evaluation of the binding activity of chimeric and humanized 4B10 monoclonal antibodies

嵌合及人類化4B10抗體係如在實例3所敘述製造及純化並分析其結合至B細胞株B104的能力,B細胞株內源地藉由FACS表現CD52。簡言之,2 x 105 B104細胞係於包含5%胎牛血清及5%羊血清的PBS中和抗體(0.02微克/毫升至16.7微克/毫升)一起培養。所結合抗體以FITC標記的羊抗-人類二級抗體(其偵測嵌合或人類化抗-CD52抗體)偵測,經標記細胞係使用FACSCalibur系統(Becton Dickinson)分析。第18圖顯示每一個正常化(經分裂)的幾何平均螢光強度較僅-2°樣品的倍數增加。用於該檢測的該11個不同濃度(於X軸的第12個點為僅二級)的人類化及嵌合抗體係示於X軸,及幾何平均倍數增加於平均螢光的幾何平均倍數增加係示於Y軸。結果顯示相較於嵌合4B10抗體,所結合人類化4B10抗體結合至CD52表現細胞的能力一樣好或些微更佳。Chimeric and Humanized 4B10 Anti-Systems As described in Example 3, the ability to bind to B cell line B104 was produced and purified and analyzed, and the B cell line endogenously expressed CD52 by FACS. Briefly, 2 x 105 B104 cells were cultured in PBS neutralizing antibody (0.02 μg/ml to 16.7 μg/ml) containing 5% fetal bovine serum and 5% goat serum. The bound antibodies were detected with FITC-labeled goat anti-human secondary antibody (which detects chimeric or humanized anti-CD52 antibodies) and the labeled cell lines were analyzed using the FACSCalibur system (Becton Dickinson). Figure 18 shows an increase in the geometric mean fluorescence intensity of each normalized (split) compared to a multiple of only -2° sample. The humanized and chimeric resistance systems for the 11 different concentrations (12th point on the X-axis are only secondary) for this assay are shown on the X-axis, and the geometric mean fold is increased by the geometric mean multiple of the mean fluorescence. The increase is shown on the Y axis. The results show that the ability of the bound humanized 4B10 antibody to bind to CD52 expressing cells is as good or slightly better than the chimeric 4B10 antibody.

實例16:嵌合及人類化4B10單株抗體ADCC活性之評估Example 16: Evaluation of ADCC activity of chimeric and humanized 4B10 monoclonal antibodies

評估嵌合及人類化4B10抗體媒介CD52-表現細胞的ADCC殺傷之能力。ADCC檢測係如在上文實例6所敘述執行。簡言之,設計為表現CD52蛋白(CHO-CD52)的CHO K1細胞係用作標的細胞並以Na251CrO4(New England Nuclear,Boston,MA)於37℃標記1-2小時。洗滌細胞,再懸浮於具10% FCS的RPMI 1640介質中,及與嵌合或人類化4B10抗體以範圍自10微克/毫升至0.01微克/毫升的各種濃度混合。人類PBMC係用作效應細胞並以1:50標的-對-效應細胞比例加入,在6小時隔夜培養之後,自每一孔收集25微升不含細胞的上層清液,並以MicroBeta Trilux閃爍計數器(Wallac,Gaithersburg,MD)計數。自發釋出的51Cr量係由單獨在介質中培養標的細胞而得到。自標的細胞的自發釋出典型上小於20%。所併入51Cr總量係由加入1%Triton X-100至蒸餾水而決定,而裂解百分率係如下計算:[(樣品c.p.m.-自發c.p.m.)/(總c.p.m.-自發c.p.m.)] X 100。The chimeric and humanized 4B10 antibody mediator CD52-expressing cells were evaluated for their ability to kill ADCC. The ADCC assay was performed as described in Example 6 above. Briefly, a CHO K1 cell line designed to express CD52 protein (CHO-CD52) was used as the target cell and labeled with Na251CrO4 (New England Nuclear, Boston, MA) for 1-2 hours at 37 °C. The cells were washed, resuspended in RPMI 1640 medium with 10% FCS, and mixed with chimeric or humanized 4B10 antibody at various concentrations ranging from 10 micrograms/ml to 0.01 micrograms/ml. Human PBMCs were used as effector cells and were added at a 1:50 standard-to-effector cell ratio. After 6 hours of overnight incubation, 25 microliters of cell-free supernatant was collected from each well and MicroBeta Trilux scintillation counter was used. (Wallac, Gaithersburg, MD) counts. The spontaneously released 51Cr amount is obtained by culturing the target cells alone in the medium. The spontaneous release of self-labeled cells is typically less than 20%. The total amount of 51Cr incorporated was determined by the addition of 1% Triton X-100 to distilled water, and the percentage of cracking was calculated as follows: [(sample c.p.m.-spontaneous c.p.m.)/(total c.p.m.-spontaneous c.p.m.)] X 100.

第19圖說明用於檢測中對照、嵌合及人類化4B10抗體的濃度(X軸),Y軸顯示%特定殺傷。結果顯示相較於嵌合4B10抗體,人類化4B10抗體媒介相當或些微更佳的ADCC殺傷。IgG1同種型對照於所測試濃度顯示僅低位準的背景殺傷。Figure 19 illustrates the concentration (X-axis) used to detect the control, chimeric, and humanized 4B10 antibodies, and the Y-axis shows % specific killing. The results show that the humanized 4B10 antibody medium is comparable or slightly better ADCC killing than the chimeric 4B10 antibody. The IgGl isotype control showed only low level background killing at the concentrations tested.

實例17:嵌合及人類化4B10單株抗體CDC活性之評估Example 17: Evaluation of chimeric and humanized 4B10 monoclonal antibody CDC activity

評估嵌合及人類化4B10抗體在人類補體存在下對內源地表現CD52的B104細胞媒介細胞毒效應之能力。使用CellTiter Glo套組(Promega)決定殘基在試驗的活細胞。簡言之,B104細胞(標的細胞)係以2.5x104細胞/孔置於96孔培養盤中,與嵌合或人類化4B10抗體以範圍自1微克/毫升至25微克/毫升的各種濃度混合,並加入人類補體至10%的最終濃度。僅補體而無抗體及僅抗體而無補體係用作對照以決定背景。在於37℃培養三小時後,以每分鐘1500轉離心培養盤3分鐘,而存在於沉澱細胞團塊的活細胞係使用CellTiter Glo分析決定。以Envision機器讀取培養盤。第20圖顯示使用CellTiter Glo分析測量的存在於試驗的活細胞。再次,隨著人類化及嵌合4B10抗體的濃度增加,活細胞數目減少。這些結果建議在B104細胞的CDC媒介殺傷中,人類化抗體較嵌合4B10抗體表現一樣好或些微更佳。The ability of chimeric and humanized 4B10 antibodies to endogenously express the cytotoxic effects of B104 cells of CD52 in the presence of human complement was assessed. The cells in the assay were determined using the CellTiter Glo kit (Promega). Briefly, B104 cells (target cells) were plated at 2.5x104 cells/well in 96-well plates and mixed with chimeric or humanized 4B10 antibodies at various concentrations ranging from 1 μg/ml to 25 μg/ml. And add human complement to a final concentration of 10%. Only complement and no antibody and only antibody and no complement system were used as controls to determine background. After three hours of incubation at 37 ° C, the plates were centrifuged at 1500 rpm for 3 minutes, while the viable cell lines present in the pellet pellets were determined using CellTiter Glo analysis. The plate was read on an Envision machine. Figure 20 shows live cells present in the assay as measured using the CellTiter Glo assay. Again, as humanization and the concentration of chimeric 4B10 antibodies increase, the number of viable cells decreases. These results suggest that humanized antibodies perform as well or slightly better than chimeric 4B10 antibodies in CDC vector killing of B104 cells.

實例18:於CD52基因轉殖老鼠中嵌合及人類化抗-CD52抗體的藥物動力數據之分析(12G6、7F11、嵌合及人類化4B10)Example 18: Analysis of drug kinetic data for chimeric and humanized anti-CD52 antibodies in CD52 transgenic mice (12G6, 7F11, chimeric and humanized 4B10)

以Campath、12G6、7F11、及嵌合及人類化4B10抗-CD52抗體其中一個投藥至人類CD52基因轉殖老鼠,以檢查淋巴細胞消耗位準。取這些抗體其中一個100微升體積,以1毫克/公斤的劑量靜脈內注射至老鼠,為分析抗-抗體反應,於抗體注射後2小時、1、2、4、7、及10天後經由眼窩後叢內穿刺收集100微升血液至血清分離管。使用ELISA分析決定每一個血清樣本中循環人類IgG1的含量。基於抗體循環位準,Campath、7F11、及4B10的嵌合及人類化形式之間存在些微或沒有任何差異。注射後12G6抗體顯現較低cmax值,其暗示此抗體可能快速退化。第21圖顯示Campath、12G6(嵌合)、7F11(嵌合)、4B10(嵌合)及4B10(人類化)抗體的藥物動力數據。Campath One of the 12G6, 7F11, and chimeric and humanized 4B10 anti-CD52 antibodies was administered to human CD52 gene transgenic mice to check the level of lymphocyte depletion. One hundred microliters of these antibodies were injected intravenously into mice at a dose of 1 mg/kg for analysis of anti-antibody reactions, 2 hours, 1, 2, 4, 7, and 10 days after antibody injection. 100 microliters of blood was collected from the posterior plexus of the orbit to the serum separation tube. ELISA analysis was used to determine the circulating human IgGl content in each serum sample. Based on antibody circulating level, Campath There is little or no difference between the chimeric and humanized forms of 7F11, and 4B10. The 12G6 antibody exhibited a lower cmax value after injection, suggesting that this antibody may degrade rapidly. Figure 21 shows Campath Drug kinetic data for 12G6 (chimeric), 7F11 (chimeric), 4B10 (chimeric) and 4B10 (humanized) antibodies.

實例19:於CD52基因轉殖老鼠中嵌合及人類化抗-CD52抗體的消耗活性之分析(嵌合及人類化4B10)Example 19: Analysis of the depletion activity of chimeric and humanized anti-CD52 antibodies in CD52 transgenic mice (chimeric and humanized 4B10)

將Campath或嵌合或人類化4B10抗-人類CD52抗體投藥至人類CD52基因轉殖老鼠,以檢查淋巴細胞消耗量。將100微升體積嵌合或人類化4B10抗-人類CD52抗體以1毫克/公斤的劑量靜脈內注射至老鼠。三天之後殺死老鼠及收集血液及脾臟以決定B及T-細胞消耗的位準。利用流式細胞計數法評估存在於huCD52基因轉殖老鼠的循環週邊血液的總T輔助細胞、細胞毒性T細胞、及B細胞之絕對數。這些淋巴細胞族群係由其下列蛋白抗原的表面表現而定義:CD4表現辨識T輔助細胞族群,CD8表現辨識細胞毒性T細胞族群及CD19表現辨識所有成熟B細胞族群。脾臟中消耗活性的比較顯示在投藥Campath或嵌合或人類化形式的4B10之後所消耗T細胞位準沒有任何差別。因為所使用的低劑量,於脾臟中觀察到僅中度位準的B細胞消耗。於每動物基準,顯然在媒介淋巴細胞消耗上人類化4B10抗體與Campath為一樣好或是些微更佳。第22A-22C圖顯示在使用嵌合及人類化抗體投藥之後72小時血液中CD4 T細胞、CD8 T細胞及CD19 B細胞的位準。Will Campath Or chimeric or humanized 4B10 anti-human CD52 antibody was administered to human CD52 gene transgenic mice to check lymphocyte consumption. One hundred microliters of chimeric or humanized 4B10 anti-human CD52 antibody was injected intravenously into mice at a dose of 1 mg/kg. After three days, the mice were killed and blood and spleen were collected to determine the level of B and T-cell consumption. The absolute number of total T helper cells, cytotoxic T cells, and B cells present in the circulating peripheral blood of huCD52 gene-transferred mice was evaluated by flow cytometry. These lymphocyte populations are defined by the surface manifestations of the following protein antigens: CD4 expression identifies T helper cell populations, CD8 expression identifies cytotoxic T cell populations, and CD19 expression recognizes all mature B cell populations. A comparison of the consuming activity in the spleen is shown in the administration of Campath There was no difference in the level of T cells consumed after 4B10 in chimeric or humanized form. Only a moderate level of B cell consumption was observed in the spleen because of the low dose used. On each animal benchmark, apparently on the media lymphocyte depletion of humanized 4B10 antibody with Campath It's as good or slightly better. Figures 22A-22C show the levels of CD4 T cells, CD8 T cells, and CD19 B cells in the blood 72 hours after administration of chimeric and humanized antibodies.

實例20:抗-人類CD52抗體的相對結合效率Example 20: Relative binding efficiency of anti-human CD52 antibodies

使用設計為表現CD52的CHO細胞評估所選擇抗-CD52抗體的EC50值。CHO-CD52細胞係於0.25%胰蛋白酶胰蛋白化,收集,及使用PBS/5% FBS潤洗。接著將細胞以每孔1E5細胞沉積至圓底96孔培養盤。初級抗體染色係使用每一個抗-CD52嵌合抗體以起始濃度50微克/毫升的12點連續稀釋(1:2)而完成。使用於10微克/毫升(Jackson 109-096-098)二級的抗-人類Fcγ的FITC-共軛羊FAB2片段,將細胞在每一次培養前及後於冰-冷PBS/5% FBS洗滌3次,將細胞固定於包含2%不含甲醇多聚甲醛的PBS及由流式細胞計數法評估,流式細胞數據係使用Graph pad Prizm軟體分析以決定95%信賴區間的EC50值。EC50 values of selected anti-CD52 antibodies were assessed using CHO cells designed to express CD52. CHO-CD52 cell line was trypsinized in 0.25% trypsin, collected, and rinsed with PBS/5% FBS. The cells were then deposited in 1E5 cells per well into round bottom 96 well plates. Primary antibody staining was done using 12-point serial dilutions (1:2) of each anti-CD52 chimeric antibody at an initial concentration of 50 micrograms/ml. The FITC-conjugated sheep FAB2 fragment of secondary anti-human Fcγ was used at 10 μg/ml (Jackson 109-096-098), and the cells were washed in ice-cold PBS/5% FBS before and after each culture. The cells were fixed in PBS containing 2% methanol-free paraformaldehyde and evaluated by flow cytometry. Flow cytometry was performed using Graph pad Prizm software analysis to determine the EC50 value of the 95% confidence interval.

結合數據(第23圖)顯示該新的CD52抗體不僅具如先前所敘述不同的抗原決定區專一性,亦具如下表所顯示不同的結合特徵。Campath-1H、7F11、4B10、2C3及12G6嵌合抗體顯示在0.5至2.5微克/毫升之間相當類似的EC 50值。9D9嵌合抗體顯示些微不同的結合特徵,其EC50值在約5至7微克/毫升。4B10人類化抗體顯示與嵌合4B10抗體類似的結合特徵,其顯示人類化抗體保留嵌合4B10抗體的結合特徵。Binding data (Fig. 23) shows that the new CD52 antibody not only has different epitope-specificity as previously described, but also has different binding characteristics as shown in the following table. Campath-1H The 7F11, 4B10, 2C3 and 12G6 chimeric antibodies showed comparable EC50 values between 0.5 and 2.5 μg/ml. The 9D9 chimeric antibody showed slightly different binding characteristics with an EC50 value of about 5 to 7 micrograms per milliliter. The 4B10 humanized antibody showed similar binding characteristics to the chimeric 4B10 antibody, which showed that the humanized antibody retained the binding characteristics of the chimeric 4B10 antibody.

C1H表示Campath-1H . C1H means Campath-1H .

實例21:抗-CD52抗體細胞株7F11的人類化Example 21: Humanization of anti-CD52 antibody cell line 7F11

抗-人類CD52抗體細胞株7F11的人類化係由自老鼠7F11抗體移植CDR區域至人類抗體變異區骨架如在實例14對4B10抗體人類化所敘述。7F11重鏈及輕鏈CDR-1、CDR-2、及CDR-3序列係分別移植至VH3-72及VK2 A18b人類骨架區。人類JH6(WGQGTTVTVSS: SEQ ID NO: 133)及JK2(FGQGTKLEIK: SEQ ID NO: 134)序列係分別選擇為人類化重鏈及輕鏈的C-端肽,以產生7F11的人類化重鏈(7F11-SFD1及7F11-SFD2)及人類化輕鏈(7F11-VK2)變異區序列(第24圖)。該兩個人類化重鏈變異區序列(7F11-SFD1及7F11-SFD2)差別在於在CDR-3區域的一個胺基酸序列.,7F11-SFD1版本在位置93是蘇胺酸(由Kabat編號系統表示),然而7F11-SFD2版本於此位置是丙胺酸,在第24圖7F11-SFD1及7F11-SFD2的位置93皆加底線。The humanized line of the anti-human CD52 antibody cell line 7F11 was constructed by grafting the CDR regions from the mouse 7F11 antibody to the human antibody variant region backbone as described in Example 14 for the humanization of the 4B10 antibody. The 7F11 heavy and light chain CDR-1, CDR-2, and CDR-3 sequences were grafted into the VH3-72 and VK2 A18b human framework regions, respectively. Human JH6 (WGQGTTVTVSS: SEQ ID NO: 133) and JK2 (FGQGTKLEIK: SEQ ID NO: 134) sequences were selected as human C-terminal peptides of heavy and light chains, respectively, to generate 7F11 humanized heavy chain (7F11) - SFD1 and 7F11-SFD2) and humanized light chain (7F11-VK2) variant region sequences (Fig. 24). The two humanized heavy chain variant region sequences (7F11-SFD1 and 7F11-SFD2) differ in an amino acid sequence in the CDR-3 region. The 7F11-SFD1 version is sulphate at position 93 (by the Kabat numbering system) Indicated), however, the 7F11-SFD2 version is alanine at this position, and the bottom line is added at position 93 of Figures 7F11-SFD1 and 7F11-SFD2.

7F11-SFD1(SEQ ID NO: 274)的全長重鏈胺基酸序列及7F11-K2(SEQ ID NO: 275)的全長輕鏈胺基酸序列係示於第107圖。The full length heavy chain amino acid sequence of 7F11-SFD1 (SEQ ID NO: 274) and the full length light chain amino acid sequence of 7F11-K2 (SEQ ID NO: 275) are shown in Figure 107.

實例22:嵌合及人類化7F11單株抗體結合活性之評估Example 22: Evaluation of chimeric and humanized 7F11 monoclonal antibody binding activity

嵌合及人類化7F11抗體(7F11-SFD1/K2及7F11-SFD2/K2)係使用在實例3所敘述方法製造及純化,並藉由流式細胞計數法分析其結合至於CHO-CD52細胞表面表現的CD52(CHO細胞係設計為表現人類CD52)之能力。簡言之,2 x 105個CHO-CD52細胞於包含5%胎牛血清及5%羊血清的PBS中與10微克/毫升的抗體一起培養。所結合抗體是以FITC標記的羊抗-人類二級抗體(其偵測嵌合或人類化抗-CD52抗體)偵測,經標記細胞係使用FACSCalibur系統(Becton Dickinson)分析及數據係使用FlowJo version 7.2軟體(Tree Star,Inc,Oregon,USA)分析。在第25圖的統計表比較使用嵌合及人類化7F11抗體所偵測的CD52含量。結果顯示所結合人類化7F11抗體較嵌合7F11抗體結合至CD52表現細胞的能力一樣好或些微更佳。The chimeric and humanized 7F11 antibodies (7F11-SFD1/K2 and 7F11-SFD2/K2) were produced and purified using the method described in Example 3, and analyzed for their binding to CHO-CD52 cell surface by flow cytometry. The ability of CD52 (the CHO cell line is designed to express human CD52). Briefly, 2 x 105 CHO-CD52 cells were incubated with 10 μg/ml of antibody in PBS containing 5% fetal bovine serum and 5% goat serum. The bound antibody is detected by FITC-labeled goat anti-human secondary antibody (which detects chimeric or humanized anti-CD52 antibody), the labeled cell line is analyzed using the FACSCalibur system (Becton Dickinson) and the data system is FlowJo version. 7.2 software (Tree Star, Inc, Oregon, USA) analysis. The statistical table in Figure 25 compares the CD52 levels detected using chimeric and humanized 7F11 antibodies. The results show that the bound humanized 7F11 antibody is as good or slightly better than the chimeric 7F11 antibody to bind to CD52 expressing cells.

實例23:抗-CD52抗體細胞株2C3的人類化Example 23: Humanization of anti-CD52 antibody cell line 2C3

抗-人類CD52抗體細胞株2C3的人類化係由自老鼠2C3抗體移植CDR區域至人類抗體變異區骨架如在實例14對細胞株4B10抗體人類化所敘述而執行。2C3重鏈及輕鏈CDR-1、CDR-2、及CDR-3序列係分別移植至VH3-72及VK2 A18b人類骨架區。人類JH6(WGQGTTVTVSS: SEQ ID NO: 133)及JK5(FGQGTRLEIK: SEQ ID NO: 135)序列係分別選擇為人類化重鏈及輕鏈的C-端肽,以產生2C3的人類化重鏈(2C3-SFD1)及輕鏈(2C3-VK1)變異區序列(第26A及B圖)。不像人類化細胞株4B10及7F11,經CDR-移植的人類化2C3抗體的結合親合性大為降低,結合親合性係由引入回復突變至經CDR-移植結構而恢復,且在限制回復突變數目為最小的目的下,以儘可能保持重新成型抗體為「人類」,由此降低致免疫性的可能性。將單一或多個回復突變併入人類化重及輕鏈變異區序列,回復突變位置(如由Kabat編號系統表示)係描述於下表10及表11。評估使用這些回復突變所產生的抗體的經回復結合親合性。三個輕鏈變異物(2C3-VK1(L46R),亦稱為2C3-VK11;2C3-VK1(Y36L-L46R),亦稱為2C3-VK12;及2C3-VK1(M4I-A19V-Y36L-Q45K-L46R),亦稱為2C3-VK13)及5個重鏈變異物(2C3-SFD1(L78V),亦稱為2C3-VH12;2C3-SFD1(G49A),亦稱為2C3-VH15;2C3-SFD1(G49A-L78V),亦稱為2C3-VH16;2C3-SFD1(L18M-G49A-L78V),亦稱為2C3-VH17;及2C3-SFD1(L18M-G42E-G49A-L78V),亦稱為2C3-VH19)係使用標準生物技術產生。經CDR-移植重鏈變異區序列2C3-SFD1及回復突變物2C3-VH12、2C3-VH15、2C3-VH16、2C3-VH17、及2C3-VH19的胺基酸序列係示於第26A圖且經回復突變胺基酸加底線及CDRs為粗體。類似地,對輕鏈序列,經CDR-移植變異區序列2C3-VK1及回復突變物2C3-VK11、2C3-VK12、及2C3-VK13係示於第26B圖且經回復突變胺基酸加底線及CDRs為粗體。The humanized line of the anti-human CD52 antibody cell line 2C3 was performed by grafting the CDR regions from the mouse 2C3 antibody to the human antibody variant region backbone as described in Example 14 for humanization of the cell line 4B10 antibody. The 2C3 heavy and light chain CDR - 1, CDR-2, and CDR-3 sequences were grafted into the VH3-72 and VK2 A18b human framework regions, respectively. Human JH6 (WGQGTTVTVSS: SEQ ID NO: 133) and JK5 (FGQGTRLEIK: SEQ ID NO: 135) sequences were selected as human C-terminal peptides of heavy and light chains, respectively, to generate 2C3 humanized heavy chains (2C3) -SFD1) and light chain (2C3-VK1) variant region sequences (Fig. 26A and B). Unlike humanized cell lines 4B10 and 7F11, the binding affinity of the CDR-grafted humanized 2C3 antibody was greatly reduced, and the binding affinity was restored by introduction of a back mutation to the CDR-grafted structure, and in response to restriction With the goal of minimizing the number of mutations, it is possible to keep the reshaped antibody as "human" as much as possible, thereby reducing the possibility of immunogenicity. Single or multiple back mutations were incorporated into the humanized heavy and light chain variant region sequences, and the position of the back mutation (as indicated by the Kabat numbering system) is described in Tables 10 and 11 below. The recovered binding affinity of the antibodies produced using these back mutations was assessed. Three light chain variants (2C3-VK1 (L46R), also known as 2C3-VK11; 2C3-VK1 (Y36L-L46R), also known as 2C3-VK12; and 2C3-VK1 (M4I-A19V-Y36L-Q45K- L46R), also known as 2C3-VK13) and 5 heavy chain variants (2C3-SFD1 (L78V), also known as 2C3-VH12; 2C3-SFD1 (G49A), also known as 2C3-VH15; 2C3-SFD1 ( G49A-L78V), also known as 2C3-VH16; 2C3-SFD1 (L18M-G49A-L78V), also known as 2C3-VH17; and 2C3-SFD1 (L18M-G42E-G49A-L78V), also known as 2C3-VH19 ) is produced using standard biotechnology. The amino acid sequence of the CDR-grafted heavy chain variant region sequence 2C3-SFD1 and the revertants 2C3-VH12, 2C3-VH15, 2C3-VH16, 2C3-VH17, and 2C3-VH19 is shown in Figure 26A and is replied. The mutated amino acid plus the bottom line and the CDRs are in bold. Similarly, for the light chain sequence, the CDR-graft variant region sequence 2C3-VK1 and the revertants 2C3-VK11, 2C3-VK12, and 2C3-VK13 are shown in Figure 26B and the back-mutated amino acid is added to the bottom line and The CDRs are in bold.

2C3-SFD1(SEQ ID NO: 272)的全長重鏈胺基酸序列及2C3-K12(SEQ ID NO: 273)的全長輕鏈胺基酸序列係示於第106圖。The full length heavy chain amino acid sequence of 2C3-SFD1 (SEQ ID NO: 272) and the full length light chain amino acid sequence of 2C3-K12 (SEQ ID NO: 273) are shown in Figure 106.

實例24:嵌合及人類化2C3單株抗體結合活性之評估Example 24: Evaluation of chimeric and humanized 2C3 monoclonal antibody binding activity

嵌合及人類化2C3抗體係使用在實例3所敘述方法製造及純化,數種由配對重鏈突變物及輕鏈突變物而產生的人類化抗體,及相對應嵌合抗體係使用在實例22所敘述方法藉由流式細胞計數法分析其結合至在CHO-CD52細胞表面表現的CD52之能力。結合數據暗示由配對重鏈變異與輕鏈變異2C3-VK1或2C3-VK11所產生的細胞株具減少的結合能力,然而由配對重鏈變異與2C3-VK12或2C3-VK13所產生的細胞株顯示與嵌合2C3抗體相當或較之為佳的結合。所選擇細胞株的代表性統計表(第27A圖)比較由嵌合及人類化2C3抗體所偵測的CD52位準。與相對應嵌合抗體相較,2C3-SFD1/K1的結合顯著降低。當與重鏈2C3-SFD1配對以製造抗體2C3-SFD1/K11時,併入單一老鼠殘基於輕鏈的位置46(白胺酸白胺酸至精胺酸)(產生2C3-VK11)不會恢復結合。而且,結合不會因併入三個回復突變於重鏈(產生2C3-VH17)以製造抗體2C3-H17/K11而恢復。然而,當2C3-SFD1重鏈與2C3-VK12配對時,其具兩個回復突變,以製造抗體2C3-SFD1/K12時,結合完全恢復,此暗示必須併入特定回復突變以恢復結合活性。第27B顯示一種證實結合為相當於嵌合2C3抗體結合的所選擇人類化細胞株的統計表。這些結果顯示2C3-VK12輕鏈中兩個胺基酸殘基的回復突變族以完全恢復抗體活性。當與幾乎任何重鏈變異配對時,在殘基36(Y至L)及46(L至R)的變化能夠恢復結合。如此,顯示具最少衍生自原始老鼠抗體的骨架殘基的經恢復結合的人類化2C3細胞株係為2C3-SFD1/K12。The chimeric and humanized 2C3 anti-systems were made and purified using the methods described in Example 3, several humanized antibodies produced by pairing heavy chain mutants and light chain mutants, and corresponding chimeric anti-systems were used in Example 22 The described method analyzes its ability to bind to CD52 expressed on the surface of CHO-CD52 cells by flow cytometry. The binding data suggests that the cell line produced by the paired heavy chain variation and the light chain variant 2C3-VK1 or 2C3-VK11 has reduced binding ability, whereas the cell line produced by paired heavy chain variation and 2C3-VK12 or 2C3-VK13 shows A comparable or better binding to the chimeric 2C3 antibody. A representative statistical table of the selected cell lines (Fig. 27A) compares the CD52 levels detected by chimeric and humanized 2C3 antibodies. The binding of 2C3-SFD1/K1 was significantly reduced compared to the corresponding chimeric antibody. When paired with heavy chain 2C3-SFD1 to make antibody 2C3-SFD1/K11, incorporation of a single mouse residue based on position 40 of the light chain (leucine to arginine) (production of 2C3-VK11) does not recover Combine. Moreover, binding was not restored by the incorporation of three back mutations to the heavy chain (which produced 2C3-VH17) to make the antibody 2C3-H17/K11. However, when the 2C3-SFD1 heavy chain was paired with 2C3-VK12, it had two back mutations to make the antibody 2C3-SFD1/K12, and the binding was completely restored, suggesting that a specific back mutation must be incorporated to restore the binding activity. Figure 27B shows a statistical table demonstrating binding to selected humanized cell lines corresponding to chimeric 2C3 antibody binding. These results show a reversion family of two amino acid residues in the 2C3-VK12 light chain to fully restore antibody activity. Changes in residues 36 (Y to L) and 46 (L to R) are able to restore binding when paired with almost any heavy chain variation. Thus, the restored binding humanized 2C3 cell line with minimal backbone residues derived from the original mouse antibody was shown to be 2C3-SFD1/K12.

實例25:抗-CD52抗體細胞株12G6的人類化Example 25: Humanization of anti-CD52 antibody cell line 12G6

抗-人類CD52抗體細胞株12G6的人類化係由自老鼠12G6抗體移植CDR區域至人類抗體變異區骨架如在實例14對細胞株4B10抗體人類化所敘述而執行。12G6重鏈及輕鏈CDR-1、CDR-2、及CDR-3序列係分別移植至VH3-72及VK2 A18b人類骨架區。人類JH6(WGQGTTVTVSS: SEQ ID NO: 133)及JK2(FGQGTKLEIK: SEQ ID NO: 134)序列係分別選擇為人類化重鏈及輕鏈的C-端肽,以產生12G6的人類化重鏈(12G6-SFD1)及輕鏈(12G6-VK1)變異區序列(第28A及28B圖)。當12G6-SFD1重鏈變異區及12G6-VK1輕鏈變異區合併於人類化12G6-SFD1/K1抗體時,CD52的結合親合性大為降低,結合親合性係由引入回復突變至經CDR-移植結構而恢復,將單一或多個回復突變併入人類化重及輕鏈變異區序列,這些回復突變的位置(如由Kabat編號系統表示)係描述於下表12及表13。評估使用這些回復突變所產生的抗體的經回復結合親合性。四個輕鏈變異(12G6-VK1(Y36V),亦稱為12G6-VK10;12G6-VK1(Y36V-Q45K-L46R),亦稱為12G6-VK11;12G6-VK1(Y36V-L46R),亦稱為12G6-VK12;及12G6-VK1(L46R),亦稱為12G6-VK13)及三個重鏈變異(12G6-SFD1(L78V),亦稱為12G6-VH10;12G6-SFD1(G49A),亦稱為12G6-VH11;及12G6-SFD1(G49A-L78V),亦稱為12G6-VH12)係使用標準分子生物技術產生。經CDR-移植重鏈變異區序列12G6-SFD1及回復突變12G6-VH10、12G6-VH11、及12G6-VH12的胺基酸序列係示於第28A圖且經回復突變胺基酸加底線及CDRs為粗體。類似地,對輕鏈序列,經CDR-移植變異區序列12G6-VK1及回復突變12G6-VH10、12G6-VH11、12G6-VK12、及12G6-VK13係示於第28B圖且經回復突變胺基酸加底線及CDRs為粗體。The humanized line of the anti-human CD52 antibody cell line 12G6 was performed by grafting the CDR regions from the mouse 12G6 antibody to the human antibody variant region backbone as described in Example 14 for humanization of the cell line 4B10 antibody. The 12G6 heavy and light chain CDR-1, CDR-2, and CDR-3 sequences were grafted into the VH3-72 and VK2 A18b human framework regions, respectively. The human JH6 (WGQGTTVTVSS: SEQ ID NO: 133) and JK2 (FGQGTKLEIK: SEQ ID NO: 134) sequences were selected as human C-terminal peptides of heavy and light chains, respectively, to generate 12G6 humanized heavy chains (12G6). -SFD1) and light chain (12G6-VK1) variant region sequences (Figs. 28A and 28B). When the 12G6-SFD1 heavy chain variant region and the 12G6-VK1 light chain variant region are combined with the humanized 12G6-SFD1/K1 antibody, the binding affinity of CD52 is greatly reduced, and the binding affinity is introduced by the back mutation to the CDR. - Recovery of the transplanted structure, incorporating single or multiple back mutations into the humanized heavy and light chain variant region sequences, the positions of these back mutations (as indicated by the Kabat numbering system) are described in Tables 12 and 13 below. The recovered binding affinity of the antibodies produced using these back mutations was assessed. Four light chain variants (12G6-VK1 (Y36V), also known as 12G6-VK10; 12G6-VK1 (Y36V-Q45K-L46R), also known as 12G6-VK11; 12G6-VK1 (Y36V-L46R), also known as 12G6-VK12; and 12G6-VK1 (L46R), also known as 12G6-VK13) and three heavy chain variants (12G6-SFD1 (L78V), also known as 12G6-VH10; 12G6-SFD1 (G49A), also known as 12G6-VH11; and 12G6-SFD1 (G49A-L78V), also known as 12G6-VH12) are produced using standard molecular biology techniques. The amino acid sequence of the CDR-grafted heavy chain variant region sequence 12G6-SFD1 and the back mutations 12G6-VH10, 12G6-VH11, and 12G6-VH12 is shown in Figure 28A and the back-mutated amino acid plus the bottom line and CDRs are Bold. Similarly, for the light chain sequence, the CDR-graft variant region sequence 12G6-VK1 and the back mutations 12G6-VH10, 12G6-VH11, 12G6-VK12, and 12G6-VK13 are shown in Figure 28B and the mutated amino acid is reverted. Bottom lines and CDRs are bold.

12G6-SFD1(SEQ ID NO: 279)的全長重鏈胺基酸序列及12G6-K12(SEQ ID NO: 280)的全長輕鏈胺基酸序列係示於第109圖。The full length heavy chain amino acid sequence of 12G6-SFD1 (SEQ ID NO: 279) and the full length light chain amino acid sequence of 12G6-K12 (SEQ ID NO: 280) are shown in Figure 109.

實例26:嵌合及人類化12G6單株抗體結合活性之評估Example 26: Evaluation of the binding activity of chimeric and humanized 12G6 monoclonal antibodies

嵌合及人類化12G6抗體係使用在實例3所敘述方法製造及純化,數種由配對重鏈變異及輕鏈變異而產生的人類化抗體,及相對應嵌合抗體,係使用在實例22所敘述方法藉由流式細胞計數法分析其結合至於CHO-CD52細胞表面表現的CD52之能力。結合數據暗示由配對重鏈變異與輕鏈變異12G6-VK1、12G6-VK10、或12G6-VK11所產生的細胞株具減少的結合能力,然而由配對重鏈變異與12G6-VK11或12G6-VK12所產生的細胞株顯示與相對應嵌合12G6抗體相當或較之為佳的結合。所選擇細胞株的代表性統計表(第29圖)比較由嵌合及人類化12G6抗體所偵測的CD52位準。這些結果顯示12G6輕鏈變異區(細胞株12G6-VK12)中兩個胺基酸殘基的回復突變足以完全恢復抗體活性。當與幾乎任何重鏈變異配對時,在Kabat編碼殘基36(Y至L)及46(L至R)的變化能夠恢復結合。如此,顯示具最少衍生自原始老鼠抗體的骨架殘基的經恢復結合的人類化212G6細胞株係為12G6-SFD1/K12。The chimeric and humanized 12G6 anti-systems were made and purified using the methods described in Example 3, several humanized antibodies produced by paired heavy chain variations and light chain variations, and corresponding chimeric antibodies were used in Example 22. The narrative method analyzes its ability to bind to CD52 expressed on the surface of CHO-CD52 cells by flow cytometry. Binding data suggest that the cell line produced by the paired heavy chain variant and the light chain variant 12G6-VK1, 12G6-VK10, or 12G6-VK11 has reduced binding capacity, whereas by paired heavy chain variation with 12G6-VK11 or 12G6-VK12 The resulting cell line shows a binding comparable or better than the corresponding chimeric 12G6 antibody. A representative statistical table of the selected cell lines (Fig. 29) compares the CD52 levels detected by chimeric and humanized 12G6 antibodies. These results show that the back mutation of the two amino acid residues in the 12G6 light chain variant region (cell line 12G6-VK12) is sufficient to fully restore antibody activity. Changes in Kabat encoding residues 36 (Y to L) and 46 (L to R) are able to restore binding when paired with almost any heavy chain variation. Thus, the restored binding humanized 212G6 cell line with minimal backbone residues derived from the original mouse antibody was shown to be 12G6-SFD1/K12.

實例27:抗-CD52抗體細胞株9D9的人類化Example 27: Humanization of anti-CD52 antibody cell line 9D9

抗-人類CD52抗體細胞株9D9的人類化係由自老鼠9D9抗體移植CDR區域至人類抗體變異區骨架如在實例14對細胞株4B10抗體人類化所敘述而執行。9D9重鏈及輕鏈的CDR-1、CDR-2、及CDR-3序列係分別移植至VH3-23及VK2 A18b人類骨架區。人類JH6(WGQGTTVTVSS:SEQ ID NO: 133)及JK2(FGQGTKLEIK:SEQ ID NO: 134)序列係分別選擇為人類化重鏈及輕鏈的C-端肽,以產生人類化重鏈(9D9-VH10)及輕鏈(9D9-VK2)變異區序列(第30A及30B圖)。當9D9-VH10重鏈變異區及9D9-VK2輕鏈變異區合併於人類化9D9-H10/K2抗體時,CD52的結合親合性大為降低,結合親合性係由引入回復突變至經CDR-移植結構而恢復,將單一或多個回復突變併入人類化重及輕鏈變異區序列,這些回復突變的位置(如由Kabat編號系統表示)係描述於下表14及表15。評估使用這些回復突變所產生的抗體的經回復結合親合性。四個輕鏈變異(9D9-VK2(Y36L-Q45K-L46R),亦稱為9D9-VK12;9D9-VK2(Y36L-L46R),亦稱為9D9-VK13;9D9-VK2(L46R),亦稱為9D9-VK14;及9D9-VK2(Q45K-L46R),亦稱為9D9-VK15)及五個重鏈變異(9D9-VH10(W47L-V48T-S49A-N76S-L78V),亦稱為9D9-VH11;9D9-VH10(W47L-V48T-S49A),亦稱為9D9-VH15;9D9-VH10(W47L),亦稱為9D9-VH16;9D9-VH10(W47L-V48T),亦稱為9D9-VH17;及9D9-VH10(W47L-S49A),亦稱為9D9-VH18)係使用標準分子生物技術產生。經CDR-移植重鏈變異區序列9D9-VH10及回復突變9D9-VH11、9D9-VH15、9D9-VH16、9D9-VH17、及9D9-VH18的胺基酸序列係示於第30A圖且經回復突變胺基酸加底線及CDRs為粗體。類似地,對輕鏈序列,經CDR-移植變異區序列9D9-VK2及回復突變9D9-VK12、9D9-VK13、9D9-VK14、及9D9-VK15係示於第30B圖且經回復突變胺基酸加底線及CDRs為粗體。The humanized line of anti-human CD52 antibody cell line 9D9 was performed by grafting the CDR regions from the mouse 9D9 antibody to the human antibody variant region backbone as described in Example 14 for humanization of the cell line 4B10 antibody. The CDR-1, CDR-2, and CDR-3 sequences of the 9D9 heavy and light chains were grafted into the VH3-23 and VK2 A18b human framework regions, respectively. The human JH6 (WGQGTTVTVSS: SEQ ID NO: 133) and JK2 (FGQGTKLEIK: SEQ ID NO: 134) sequences were selected as human C-terminal peptides of heavy and light chains, respectively, to generate humanized heavy chains (9D9-VH10). And the light chain (9D9-VK2) variant region sequence (Figs. 30A and 30B). When the 9D9-VH10 heavy chain variant region and the 9D9-VK2 light chain variant region are combined with the humanized 9D9-H10/K2 antibody, the binding affinity of CD52 is greatly reduced, and the binding affinity is introduced by the back mutation to the CDR. - Recovery of the transplanted structure, incorporating single or multiple back mutations into the humanized heavy and light chain variant region sequences, the positions of these back mutations (as indicated by the Kabat numbering system) are described in Tables 14 and 15 below. The recovered binding affinity of the antibodies produced using these back mutations was assessed. Four light chain variants (9D9-VK2 (Y36L-Q45K-L46R), also known as 9D9-VK12; 9D9-VK2 (Y36L-L46R), also known as 9D9-VK13; 9D9-VK2 (L46R), also known as 9D9-VK14; and 9D9-VK2 (Q45K-L46R), also known as 9D9-VK15) and five heavy chain variants (9D9-VH10 (W47L-V48T-S49A-N76S-L78V), also known as 9D9-VH11; 9D9-VH10 (W47L-V48T-S49A), also known as 9D9-VH15; 9D9-VH10 (W47L), also known as 9D9-VH16; 9D9-VH10 (W47L-V48T), also known as 9D9-VH17; and 9D9 -VH10 (W47L-S49A), also known as 9D9-VH18) is produced using standard molecular biology techniques. The amino acid sequence of the CDR-grafted heavy chain variant region sequence 9D9-VH10 and the back mutations 9D9-VH11, 9D9-VH15, 9D9-VH16, 9D9-VH17, and 9D9-VH18 is shown in Figure 30A and is back-mutated. The amino acid bottom line and CDRs are in bold. Similarly, for the light chain sequence, the CDR-graft variant region sequence 9D9-VK2 and the back mutations 9D9-VK12, 9D9-VK13, 9D9-VK14, and 9D9-VK15 are shown in Figure 30B and the mutated amino acid is reverted. Bottom lines and CDRs are bold.

9D9-H16(SEQ ID NO: 276)及9D9-H18(SEQ ID NO: 277)的全長重鏈胺基酸序列,及9D9-K13(SEQ ID NO: 278)的全長輕鏈胺基酸序列係示於第108圖。The full length heavy chain amino acid sequence of 9D9-H16 (SEQ ID NO: 276) and 9D9-H18 (SEQ ID NO: 277), and the full length light chain amino acid sequence of 9D9-K13 (SEQ ID NO: 278) Shown in Figure 108.

實例28:嵌合及人類化9D9單株抗體結合活性之評估Example 28: Evaluation of chimeric and humanized 9D9 monoclonal antibody binding activity

嵌合及人類化9D9抗體係使用在實例3所敘述方法製造及純化,數種由配對重鏈變異及輕鏈變異而產生的人類化抗體,及相對應嵌合抗體,係使用在實例22所敘述方法藉由流式細胞計數法分析其結合至於CHO-CD52細胞(CHO細胞係設計為表現人類CD52)表面表現的CD52之能力。結合數據暗示由配對重鏈變異與輕鏈變異9D9-VK2、9D9-VK14、或9D9-VK15所產生的細胞株具減少的結合能力,然而由配對9D9-VK12或9D9-VK13輕鏈變異與經回復突變重鏈變異9D9-VH11、9D9-VH15、9D9-VH16、及9D9-VH18所產生的細胞株顯示與嵌合9D9抗體相當或較之為佳的結合。當輕鏈變異9D9-VK12及9D9-VK13與母體經CDR移植重鏈9D9-VH10或經回復突變9D9-VH17序列配對時,結合顯著降低,暗示對人類化9D9細胞株,重鏈及輕鏈序列皆必須設計具回復突變以恢復結合能力。所選擇細胞株的代表性統計表(第31圖)比較由嵌合及人類化9D9抗體所偵測的CD52位準。這些結果顯示在9D91輕鏈變異區(細胞株9D9-VK13)兩個胺基酸殘基(例如,Y至L於位置36,及L至R於位置46)的回復突變為必要的以恢復抗體專一性,當與在一個位置(例如,W至L,於位置47)或在兩個位置(例如,W至L於位置47及S至A於位置49)突變的重鏈配對時。如此,顯示具最少衍生自原始老鼠抗體的骨架殘基的經恢復結合的人類化9D9細胞株係為9D9-H16/K13及9D9-H18/K13。The chimeric and humanized 9D9 anti-systems were made and purified using the methods described in Example 3, several humanized antibodies produced by paired heavy chain variations and light chain variations, and corresponding chimeric antibodies were used in Example 22 The narrative method analyzes its ability to bind to CD52 on the surface of CHO-CD52 cells (the CHO cell line is designed to express human CD52) by flow cytometry. Binding data suggest that the cell line produced by the paired heavy chain variant and the light chain variant 9D9-VK2, 9D9-VK14, or 9D9-VK15 has reduced binding ability, however, by pairing 9D9-VK12 or 9D9-VK13 light chain variation and The cell lines produced by the back-mutation heavy chain variants 9D9-VH11, 9D9-VH15, 9D9-VH16, and 9D9-VH18 showed comparable or better binding to the chimeric 9D9 antibody. When the light chain variants 9D9-VK12 and 9D9-VK13 were paired with the parental CDR-grafted heavy chain 9D9-VH10 or the back-mutated 9D9-VH17 sequence, the binding was significantly reduced, suggesting that the humanized 9D9 cell line, heavy and light chain sequences Both must be designed with a back mutation to restore binding capacity. A representative statistical table of the selected cell lines (Fig. 31) compares the CD52 levels detected by chimeric and humanized 9D9 antibodies. These results show that a back mutation of two amino acid residues (eg, Y to L at position 36, and L to R at position 46) in the 9D91 light chain variant region (cell line 9D9-VK13) is necessary to restore antibodies Specificity when paired with a heavy chain that mutates at one position (eg, W to L, at position 47) or at two positions (eg, W to L at position 47 and S to A at position 49). Thus, the restored binding humanized 9D9 cell lines with minimal backbone residues derived from the original mouse antibody were shown to be 9D9-H16/K13 and 9D9-H18/K13.

實例29:人類化抗-人類CD52抗體的相對結合效率之決定Example 29: Determination of the relative binding efficiency of humanized anti-human CD52 antibodies

嵌合及人類化抗-CD52抗體的EC50值係使用得自自商業來源(Bioreclamation,NY,USA)所提供健康捐贈者分離的CD4+ T細胞估計,CD4+ T細胞係使用EasySep套組(Stem Cell Technologies)藉由負面篩選而分離。由huCD52基因轉殖CD1老鼠脾臟細胞分離的CD4+ T細胞亦可根據在實例20對CHO-CD52細胞所敘述方法使用(幹細胞計數法)。簡言之,人類CD4+T細胞係得自健康捐贈者(Bioreclamation)的50毫升週邊血液分離,及huCD52基因轉殖老鼠CD4+T細胞係自脾臟組織分離,將細胞以PBS/5% FBS潤洗及以每孔1x105細胞沉積至圓底96孔培養盤。初級抗體染色係使用每一個抗-CD52嵌合及人類化抗體以起始濃度100微克/毫升的8點連續稀釋(1:3)而完成。使用於10微克/毫升(Jackson 109-096-098)二級抗體的抗-人類Fcγ的FITC-共軛羊F(ab')2片段,將細胞在每一次培養前及後於冰-冷PBS/5% FBS洗滌3次,將細胞固定於包含2%不含甲醇多聚甲醛的PBS及以流式細胞計數法評估,流式細胞數據係使用Graph pad Prizm軟體分析以決定95%信賴區間的EC50值。基於抗-CD52抗體至由人類PBMCS分離的CD4+T細胞及至由人類CD52基因轉殖老鼠分離的CD4+T細胞之結合,得到結合曲線(第32A、32B、32C圖)及估計EC50值及示於第33圖,所有抗體顯示至人類CD4+T細胞及至由人類CD52基因轉殖老鼠分離的CD4+T細胞的類似結合特性。結合數據顯示人類化抗體具與母體嵌合抗體相當或更佳的結合親合性,此暗示在人類化時結合親合性經保留或改善。人類化2C3及12G6抗體具較Campath-1H抗體低至少兩倍的EC50值,如由此細胞結合分析所決定。EC50 values for chimeric and humanized anti-CD52 antibodies were estimated using CD4+ T cells isolated from healthy donors from commercial sources (Bioreclamation, NY, USA), and the EasySep kit was used for CD4+ T cell lines (Stem Cell Technologies) ) Separated by negative screening. CD4+ T cells isolated from spleen cells of CD1 mouse mutated by huCD52 gene can also be used according to the method described for CHO-CD52 cells in Example 20 (stem cell counting method). Briefly, the human CD4+ T cell line was isolated from 50 ml peripheral blood of a healthy donor (Bioreclamation), and the huCD52 gene transgenic mouse CD4+ T cell line was isolated from spleen tissue, and the cells were PBS/5% FBS. and washed 1x10 5 cells per well in round-bottom 96-well culture deposited to a disk. Primary antibody staining was done using an 8-point serial dilution (1:3) of each anti-CD52 chimeric and humanized antibody at an initial concentration of 100 micrograms per milliliter. Anti-human Fcγ-based FITC-conjugated sheep F(ab') 2 fragment of 10 μg/ml (Jackson 109-096-098) secondary antibody, cells were incubated in ice-cold PBS before and after each incubation /5% FBS was washed 3 times, cells were fixed in PBS containing 2% methanol-free paraformaldehyde and evaluated by flow cytometry. Flow cytometry was performed using Graph pad Prizm software analysis to determine the 95% confidence interval. EC50 value. Based on the binding of anti-CD52 antibodies to CD4+ T cells isolated from human PBMC S and to CD4+ T cells isolated from human CD52 gene transgenic mice, binding curves (32A, 32B, 32C) and estimated EC 50 values were obtained. And as shown in Figure 33, all antibodies showed similar binding properties to human CD4+ T cells and to CD4+ T cells isolated from human CD52 gene transgenic mice. The binding data shows that the humanized antibody has comparable or better binding affinity to the parent chimeric antibody, suggesting that the binding affinity is retained or improved upon humanization. Humanized 2C3 and 12G6 antibodies are more than Campath-1H Antibodies is at least twice the EC 50 value, as determined by binding assay whereby cells.

實例30:結合人類化抗-CD52抗體至經定義之淋巴細胞族群的評估Example 30: Evaluation of binding of a humanized anti-CD52 antibody to a defined lymphocyte population

使用於以上實例7針對嵌合抗-CD52抗體所敘述的方法來評估正常提供者PBMCs中Campath-1H(C1H)及人類化2C3(2C3-SFD1/K12)、9D9(9D9-H16/K13及9D9-H18/K13)、及12G6(12G6-SFD1/K11、12G6-SFD1/K12)抗體之結合至各種PBMC子集。使用多種螢光染劑共軛抗體進行流式細胞分析。抗-CD27-PE、抗-CD19及抗-CD11c-PE Cy5、抗-CD56及抗-CD123-PE Cy7、抗-CD16-APC Cy7、及CD4-APC係得自BD Biosciences(San Diego,CA),而抗-CD54RA-ECD及抗-HLA-DR-ECD係得自Beckman Coulter。抗-CD3-太平洋藍、抗-CD8及抗-CD14-太平洋橙、及抗-CD4-APC cy5.5係得自Invitrogen(CA)。所有人類化抗-人類CD52抗體(9D9-H18/K13、9D9-H16/K13、12G6-SFD1/K11、12G6-SFD1/K12、及2C3-SFD1/K12)與Campath-1H都共軛至FITC。健康人類週邊血液單核細胞係得自冷藏保存白血球衣或是得自來自於商業廠商(Bioreclamation,NY,USA)所提供之正常捐贈者的血液所分離的單核細胞,如同在以上實例7所敘述的。為進行單核細胞的增長,使用無菌磷酸生理食鹽水(PBS)以1:1稀釋人類週邊血液及小心地分層置於聚蔗糖-泛影葡胺(GE Healthcare Bio-Sciences,Uppsala,Sweden)上,並於室溫離心30分鐘。抽出單核細胞的中間相層並於包含5%胎牛血清(FACS緩衝液)的PBS中沖洗,汙染的紅血球細胞(RBCs)以RBC裂解溶液(Sigma,St. Louis,MO,USA)裂解。將細胞再懸浮於冷的FACS緩衝液及使用40微米過濾器移除碎屑。執行多色流式細胞分析以評估人類化抗-人類CD52抗體2C3(2C3-SFD1/K12)、9D9(9D9-H16/K13及9D9-H18/K13)及12G6(12G6-SFD1/K11及12G6-SFD1/K12)相較於Campath-1H的結合能力。The method described in Example 7 above for chimeric anti-CD52 antibodies was used to assess Campath-1H in normal provider PBMCs. (C1H) and humanized 2C3 (2C3-SFD1/K12), 9D9 (9D9-H16/K13 and 9D9-H18/K13), and 12G6 (12G6-SFD1/K11, 12G6-SFD1/K12) antibodies bind to various A subset of PBMC. Flow cytometric analysis was performed using a variety of fluorescent dye conjugated antibodies. Anti-CD27-PE, anti-CD19 and anti-CD11c-PE Cy5, anti-CD56 and anti-CD123-PE Cy7, anti-CD16-APC Cy7, and CD4-APC were obtained from BD Biosciences (San Diego, CA). The anti-CD54RA-ECD and anti-HLA-DR-ECD lines were obtained from Beckman Coulter. Anti-CD3-Pacific Blue, anti-CD8 and anti-CD14-Pacific Orange, and anti-CD4-APC cy5.5 lines were obtained from Invitrogen (CA). All humanized anti-human CD52 antibodies (9D9-H18/K13, 9D9-H16/K13, 12G6-SFD1/K11, 12G6-SFD1/K12, and 2C3-SFD1/K12) with Campath-1H Both are conjugated to FITC. Healthy human peripheral blood mononuclear cell lines were obtained from cryopreserved white blood jerseys or mononuclear cells isolated from the blood of normal donors supplied by commercial manufacturers (Bioreclamation, NY, USA), as in Example 7 above. Narrated. For mononuclear cell growth, human peripheral blood was diluted 1:1 with sterile phosphate saline (PBS) and carefully layered in Ficoll-Glyceramide (GE Healthcare Bio-Sciences, Uppsala, Sweden) Top and centrifuge at room temperature for 30 minutes. The mesophase layer of monocytes was extracted and washed in PBS containing 5% fetal bovine serum (FACS buffer), and contaminated red blood cells (RBCs) were lysed with RBC lysis solution (Sigma, St. Louis, MO, USA). The cells were resuspended in cold FACS buffer and debris was removed using a 40 micron filter. Multicolor flow cytometry was performed to evaluate humanized anti-human CD52 antibodies 2C3 (2C3-SFD1/K12), 9D9 (9D9-H16/K13 and 9D9-H18/K13) and 12G6 (12G6-SFD1/K11 and 12G6-) SFD1/K12) compared to Campath-1H The ability to combine.

簡言之,1 x 106 PBMCs於FACS緩衝液的重複物使用抗體的預先-滴定稀釋液之混合物培養,以檢查淋巴細胞或骨髓樣的衍生細胞。淋巴細胞混合物包含對CD3、CD27、CD45RA、CD56、CD19、CD8、CD4、及CD16的抗體。抗體混合物係定義骨髓細胞族群,其包含對HLA-DR、CD11c、CD123、CD4、及CD14的抗體。在每一個混合物中,抗-CD52抗體中的一個以10微克/毫升得濃度培養,將細胞於4℃染色30分鐘,並沖洗及固定於包含1%多聚甲醛的PBS。100,000個染色細胞於BD LSR-I[流式細胞儀(BD Biosciences,San Jose,CA)上得到,及使用FlowJo 7.2版軟體(Tree Star,Inc,Oregan,USA)分析數據。具不同表現型特徵的多個子集已在B及T淋巴細胞之間被定義,且已顯示CD52被表現於所有人類淋巴細胞。執行多色流式細胞分析以辨識淋巴細胞子集,及以評估人類化抗-CD52抗體與在所定義子集上細胞表面CD52的結合特徵之相似點及不同點。使用標記組合,先定義出對應於B、T、NK及抗原存在細胞系的表現型不同細胞族群。評估對應於人類化抗-CD52抗體偵測於每一個經定義細胞族群上CD52表現的能力之染色強度,並將其與Campath-1H染色強度相較。統計表(第34圖)比較由在個別族群上每一個抗體所偵測的CD52程度,結果顯示所有人類化抗-CD52抗體以類似程度結合至細胞表面CD52。而且,在Campath-1H及人類化抗-CD52抗體之間在細胞表面CD52偵測位準方面沒有觀察到任何差別。於六個不同供體上執行分析,使用衍生自一個供體的細胞所產生的代表性數據示於第34圖,使用自其他供體的細胞觀察到類似結合形式。Briefly, 1 x 10 6 PBMCs were cultured in a mixture of FACS buffer replicates using a mixture of pre-titration dilutions of antibodies to examine lymphocyte or bone marrow-derived cells. The lymphocyte mixture contains antibodies to CD3, CD27, CD45RA, CD56, CD19, CD8, CD4, and CD16. The antibody mixture defines a population of myeloid cells comprising antibodies to HLA-DR, CD11c, CD123, CD4, and CD14. In each of the mixtures, one of the anti-CD52 antibodies was cultured at a concentration of 10 μg/ml, and the cells were stained at 4 ° C for 30 minutes, and washed and fixed in PBS containing 1% paraformaldehyde. 100,000 stained cells were obtained on BD LSR-I [flow cytometry (BD Biosciences, San Jose, CA) and data were analyzed using FlowJo version 7.2 software (Tree Star, Inc, Oregan, USA). Multiple subsets with different phenotypic characteristics have been defined between B and T lymphocytes, and CD52 has been shown to be expressed in all human lymphocytes. Multicolor flow cytometry was performed to identify subsets of lymphocytes, and to assess similarities and differences in the binding characteristics of humanized anti-CD52 antibodies to cell surface CD52 on defined subsets. Using a combination of markers, a population of different phenotypes corresponding to B, T, NK, and antigen-existing cell lines is first defined. To assess the staining intensity corresponding to the ability of the humanized anti-CD52 antibody to detect CD52 expression on each defined cell population, and to correlate it with Campath-1H The dyeing intensity is comparable. The statistical table (Fig. 34) compares the extent of CD52 detected by each antibody on individual populations and the results show that all humanized anti-CD52 antibodies bind to cell surface CD52 to a similar extent. Also, at Campath-1H No differences were observed between the humanized anti-CD52 antibodies on the cell surface CD52 detection level. Analysis was performed on six different donors, representative data generated using cells derived from one donor is shown in Figure 34, and similar binding formats were observed using cells from other donors.

實例31:嵌合及人類化7F11單株抗體ADCC活性之評估Example 31: Evaluation of ADCC activity of chimeric and humanized 7F11 monoclonal antibodies

評估人類化及嵌合7F11抗體於媒介CD52表現細胞的ADCC殺傷之能力。ADCC試驗係使用如在上文實例6所敘述的方法執行。簡言之,設計為表現CD52蛋白(CHO-CD52)的CHO K1細胞係被用來做為標的細胞,該標的細胞以Na2 51CrO4(New Engl㊣and Nuclear,Boston,MA)於37℃標記2-3小時。沖洗該細胞,將其懸浮於具10% FCS的RPMI 1640介質,並與IgG控制抗體、嵌合7F11抗體、或人類化7F11抗體(7F11-SFD1/K2或7F11-SFD2/K2)以範圍自5微克/毫升至0.01微克/毫升的各種濃度混合。使用NK細胞分離套組(Stem Cell Technologies)自PBMCs分離的人類NK細胞被用來做為效應細胞,並以1:5標的-對-效應細胞之比例加入。在2-6小時培養之後,自每一孔收集25微升不含細胞上層清液及於MicroBeta Trilux閃爍計數器(Wallac,Gaithersburg,MD)計數。自發釋出的51Cr的量係由單獨在介質中培養的標的細胞得到。自標的細胞的自發釋出典型地小於20%。所併入51Cr總量係由加入於蒸餾水中的1%Triton X-100而決定,而裂解百分率係如下計算:[(樣品c.p.m.-自發c.p.m.)/(總c.p.m.-自發c.p.m.)]X 100。第35圖說明用於試驗中對照IgG、嵌合7F11抗體、及人類化7F11抗體的濃度(X軸)相對於%特定裂解(Y軸)。結果顯示人類化7F11抗體(7F11-SFD1/K2及7F11-SFD2/K2)媒介較嵌合7F11抗體相當或些微更佳的ADCC殺傷。對照IgGl同種型抗體於所測試濃度顯示僅低位準的背景殺傷。The ability of humanized and chimeric 7F11 antibodies to mediate ADCC killing in vehicle CD52 was assessed. The ADCC test was performed using the method as described in Example 6 above. Briefly, a CHO K1 cell line designed to express the CD52 protein (CHO-CD52) was used as the target cell with Na 2 51 CrO 4 (New Engl plus and Nuclear, Boston, MA) at 37 ° C. Mark for 2-3 hours. The cells were washed, suspended in RPMI 1640 medium with 10% FCS, and IgG control antibody, chimeric 7F11 antibody, or humanized 7F11 antibody (7F11-SFD1/K2 or 7F11-SFD2/K2) ranging from 5 Mix at various concentrations from micrograms/ml to 0.01 micrograms/ml. Human NK cells isolated from PBMCs using the NK cell isolation kit (Stem Cell Technologies) were used as effector cells and added at a ratio of 1:5-pair-effector cells. After 2-6 hours of incubation, 25 microliters of the supernatant-free supernatant was collected from each well and counted in a MicroBeta Trilux scintillation counter (Wallac, Gaithersburg, MD). The amount of spontaneously released 51 Cr is obtained from the target cells cultured alone in the medium. The spontaneous release of self-labeled cells is typically less than 20%. The total amount of 51 Cr incorporated was determined by 1% Triton X-100 added to distilled water, and the percentage of cleavage was calculated as follows: [(sample cpm-spontaneous cpm) / (total cpm-spontaneous cpm)] X 100. Figure 35 illustrates the concentration (X-axis) versus % specific lysis (Y-axis) of the control IgG, chimeric 7F11 antibody, and humanized 7F11 antibody used in the assay. The results show that the humanized 7F11 antibody (7F11-SFD1/K2 and 7F11-SFD2/K2) vectors are comparable or slightly better ADCC killing than the chimeric 7F11 antibody. Control IgGl isotype antibodies showed only low level background killing at the concentrations tested.

實例32:嵌合及人類化7F11單株抗體CDC活性之評估Example 32: Evaluation of CDC activity of chimeric and humanized 7F11 monoclonal antibodies

評估人類化及嵌合7F11抗體於媒介CD52-表現細胞的補體依賴細胞毒性(CDC)之能力。CDC試驗係使用如在上文實例5對嵌合抗-CD52抗體所敘述的方法執行。簡言之,設計為表現CD52蛋白(CHO-CD52)的CHO K1細胞被用來做為標的細胞,並以Na2 51CrO4(New England Nuclear,Boston,MA)於37℃標記2-3小時。沖洗該細胞,將其懸浮於RPMI1640介質,並與IgG控制抗體、嵌合7F11抗體、或人類化7F11抗體(7F11-SFD1/K2或7F11-SFD2/K2)以範圍自20微克/毫升至500奈克/毫升的各種濃度混合。加入人類捕體(Sigma)至實驗孔至達到10%的最終濃度。在1-5小時培養之後,自每一孔收集25微升不含細胞上層清液並於MicroBeta Trilux閃爍計數器(Wallac,Gaithersburg,MD)計數。自發釋出的51Cr的量係自單獨在介質中培養的標的細胞得到。自標的細胞的自發釋出典型地小於20%。所併入51Cr總量係由加入於蒸餾水中的1% Triton X-100而決定,且裂解百分率係如下計算:[(每分鐘樣品計數(c.p.m.)-自發c.p.m.)/(總c.p.m.-自發c.p.m.)]X 100。第36圖說明用於試驗中對照IgG、嵌合7F11抗體、及人類化7F11抗體(7F11-SFD1/K2及7F11-SFD2/K2)的濃度(X軸)相對於%特定裂解(Y軸)。結果顯示嵌合7F11抗體與人類化抗體7F11-SFD1/K2媒介相當的殺傷,然而人類化抗體7F11-SFD2/K2媒介較嵌合7F11抗體顯著更佳的CDC殺傷。對照IgG1同種型抗體於所測試濃度顯示僅低位準的背景殺傷。The ability of humanized and chimeric 7F11 antibodies to mediate complement dependent cytotoxicity (CDC) of CD52-expressing cells was assessed. The CDC assay was performed using the method described for the chimeric anti-CD52 antibody in Example 5 above. Briefly, a protein designed to exhibit CD52 (CHO-CD52) in CHO K1 cells were used as target cells, and labeled for 2-3 hours in Na 2 51 CrO 4 (New England Nuclear, Boston, MA) at 37 [deg.] C . Rinse the cells, suspend them in RPMI1640 medium, and IgG control antibody, chimeric 7F11 antibody, or humanized 7F11 antibody (7F11-SFD1/K2 or 7F11-SFD2/K2) ranging from 20 μg/ml to 500 ng. Mix in various concentrations of grams per milliliter. Human traps (Sigma) were added to the experimental wells to a final concentration of 10%. After 1-5 hours of incubation, 25 microliters of cell free supernatant was collected from each well and counted in a MicroBeta Trilux scintillation counter (Wallac, Gaithersburg, MD). The amount of spontaneously released 51 Cr was obtained from the target cells cultured alone in the medium. The spontaneous release of self-labeled cells is typically less than 20%. The total amount of 51 Cr incorporated was determined by 1% Triton X-100 added to distilled water, and the percentage of lysis was calculated as follows: [(sample per minute (cpm) - spontaneous cpm) / (total cpm - spontaneous cpm) )] X 100. Figure 36 illustrates the concentration (X-axis) versus % specific lysis (Y-axis) for the control IgG, chimeric 7F11 antibody, and humanized 7F11 antibody (7F11-SFD1/K2 and 7F11-SFD2/K2) used in the assay. The results showed that the chimeric 7F11 antibody was comparable to the humanized antibody 7F11-SFD1/K2 vector, whereas the humanized antibody 7F11-SFD2/K2 media showed significantly better CDC killing than the chimeric 7F11 antibody. Control IgGl isotype antibodies showed only low level background killing at the concentrations tested.

實例33:嵌合及人類化2C3單株抗體ADCC活性之評估Example 33: Evaluation of ADCC activity of chimeric and humanized 2C3 monoclonal antibodies

評估人類化及嵌合2C3抗體於媒介CD52表現細胞的ADCC殺傷之能力。ADCC試驗係使用如在上文實例6所敘述的方法加以些微修改而執行。簡言之,使用CD4+T細胞分離套組(Stem Cell Technologies)自健康捐贈者PBMCs分離的T細胞被用來做為標的細胞,該標的細胞以Na2 51CrO4(New England Nuclear,Boston,MA)於37℃過夜標記2-3小時。沖洗該細胞,將其懸浮於具10% FCS的RPMI 1640介質,並與IgG控制抗體、嵌合2C3抗體、或人類化2C3抗體(2C3-SFD1/K12)以範圍自10微克/毫升至100微微克/毫升的各種濃度混合,自PBMCs分離的人類NK細胞(使用Stem Cell Technologies的NK細胞分離套組)被用來做為效應細胞,並以1:5標的-對-效應細胞的比例加入。在2-6小時培養之後,自每一孔收集25微升不含細胞上層清液及於MicroBeta Trilux閃爍計數器(Wallac,Gaithersburg,MD)計數。自發釋出的51Cr的量係自單獨在介質中培養標的細胞得到。自標的細胞的自發釋出典型地小於20%,所併入51Cr總量係由加入於蒸餾水中的1%Triton X-100而決定,且裂解百分率係如下計算:[(樣品c.p.m.-自發c.p.m.)/(總c.p.m.-自發c.p.m.)] X 100。第37圖說明用於試驗中對照IgG、嵌合2C3抗體、及人類化2C3抗體(2C3-SFD1/K12)的濃度(X軸)相對於%特定裂解(Y軸)。結果顯示人類化2C3抗體2C3-SFD1/K12媒介較2C3嵌合抗體相當的ADCC殺傷。IgG1同種型對照物於所測試濃度顯示僅低位準的背景殺傷。The ability of humanized and chimeric 2C3 antibodies to mediate ADCC killing of cells in vehicle CD52 was assessed. The ADCC test was performed using minor modifications as described in Example 6 above. Briefly, T cells isolated from healthy donor PBMCs using the CD4+ T cell isolation kit (Stem Cell Technologies) were used as target cells with Na 2 51 CrO 4 (New England Nuclear, Boston, MA) was labeled overnight at 37 ° C for 2-3 hours. The cells were washed, suspended in RPMI 1640 medium with 10% FCS, and IgG control antibody, chimeric 2C3 antibody, or humanized 2C3 antibody (2C3-SFD1/K12) ranging from 10 μg/ml to 100 pico Human NK cells isolated from PBMCs (using the NK cell isolation kit from Stem Cell Technologies) were used as effector cells at various concentrations in grams per milliliter and were added at a 1:5 target-to-effector ratio. After 2-6 hours of incubation, 25 microliters of the supernatant-free supernatant was collected from each well and counted in a MicroBeta Trilux scintillation counter (Wallac, Gaithersburg, MD). An amount of 51 Cr released spontaneously from separate lines in culture media to obtain target cells. The spontaneous release of self-labeled cells is typically less than 20%, and the total amount of 51 Cr incorporated is determined by 1% Triton X-100 added to distilled water, and the percent lysis is calculated as follows: [(sample cpm-spontaneous cpm) ) / (total cpm - spontaneous cpm)] X 100. Figure 37 illustrates the concentration (X-axis) versus % specific lysis (Y-axis) of the control IgG, chimeric 2C3 antibody, and humanized 2C3 antibody (2C3-SFD1/K12) used in the assay. The results showed that the humanized 2C3 antibody 2C3-SFD1/K12 mediator was comparable to the 2C3 chimeric antibody in ADCC killing. The IgGl isotype control showed only low level background killing at the concentrations tested.

實例34:嵌合及人類化2C3單株抗體CDC活性之評估Example 34: Evaluation of chimeric and humanized 2C3 monoclonal antibody CDC activity

評估人類化及嵌合2C3抗體於媒介CD52表現細胞的補體依賴細胞毒性(CDC)之能力。CDC試驗係使用如在上文實例5所敘述方法加以些微修改而執行。簡言之,自健康捐贈者PBMCs分離的T細胞被用來做為標的細胞,並以Na2 51CrO4(New England Nuclear,Boston,MA)於37℃過夜標記。過夜標記之後,沖洗該細胞,將其懸浮於包含10%FCS的RPMI 1640介質,並與IgG控制抗體、嵌合2C3抗體、或人類化2C3抗體(2C3-SFD1/K12)以範圍自10微克/毫升至10奈克/毫升的各種濃度混合。加入人類捕體(Sigma)至實驗孔至達到10%的最終濃度。在1-5小時培養之後,自每一孔收集25微升不含細胞上層清液並於MicroBeta Trilux閃爍計數器(Wallac,Gaithersburg,MD)計數。自發釋出的51Cr的量係自單獨在介質中培養的標的細胞得到。自標的細胞的自發釋出典型地小於20%。所併入51Cr總量係由加入於蒸餾水中1% Triton X-100而決定,且裂解百分率係如下計算:[(每分鐘樣品計數(c.p.m.)-自發c.p.m.)/(總c.p.m.-自發c.p.m.)] X 100。第38圖說明用於試驗中對照IgG、嵌合2C3抗體、及人類化2C3抗體(2C3-SFD1/K12)的濃度(X軸)相對於%特定裂解(Y軸)。結果顯示嵌合2C3抗體及人類化2C3抗體(2C3-SFD1/K12)媒介相當的裂解。對照IgG1同種型抗體於所測試濃度顯示僅低位準的背景殺傷。The ability of humanized and chimeric 2C3 antibodies to express complement-dependent cytotoxicity (CDC) of cells in vehicle CD52 was assessed. The CDC test was performed using minor modifications as described in Example 5 above. Briefly, T cells isolated from healthy donor PBMCs were used as target cells and labeled with Na 2 51 CrO 4 (New England Nuclear, Boston, MA) overnight at 37 °C. After overnight labeling, the cells were washed, suspended in RPMI 1640 medium containing 10% FCS, and IgG control antibody, chimeric 2C3 antibody, or humanized 2C3 antibody (2C3-SFD1/K12) ranging from 10 μg/ Mix in various concentrations from ML to 10 ng/ml. Human traps (Sigma) were added to the experimental wells to a final concentration of 10%. After 1-5 hours of incubation, 25 microliters of cell free supernatant was collected from each well and counted in a MicroBeta Trilux scintillation counter (Wallac, Gaithersburg, MD). The amount of spontaneously released 51 Cr was obtained from the target cells cultured alone in the medium. The spontaneous release of self-labeled cells is typically less than 20%. The total amount of 51 Cr incorporated was determined by addition of 1% Triton X-100 in distilled water, and the percentage of lysis was calculated as follows: [(sample per minute (cpm) - spontaneous cpm) / (total cpm - spontaneous cpm) ] X 100. Figure 38 illustrates the concentration (X-axis) versus % specific lysis (Y-axis) for the control IgG, chimeric 2C3 antibody, and humanized 2C3 antibody (2C3-SFD1/K12) used in the assay. The results showed that the chimeric 2C3 antibody and the humanized 2C3 antibody (2C3-SFD1/K12) media were equivalently cleaved. Control IgGl isotype antibodies showed only low level background killing at the concentrations tested.

實例35:嵌合及人類化12G6單株抗體ADCC活性之評估Example 35: Evaluation of ADCC activity of chimeric and humanized 12G6 monoclonal antibodies

評估人類化及嵌合12G6抗體於媒介CD52表現細胞的ADCC殺傷之能力。ADCC試驗係使用如在上文實例31所敘述的方法,使用自健康捐贈者PBMCs分離的T細胞做為標的細胞並藉由鉻釋出試驗而執行。第39圖說明用於此試驗中對照IgG、嵌合12G6抗體、及人類化12G6抗體(12G6-SFD1/K11或12G6-SFD1/K12)的濃度(X軸)相對於%特定裂解(Y軸)。結果顯示人類化12G6抗體12G6-SFD1/K11及12G6-SFD1/K12媒介與12G6嵌合抗體相當的ADCC殺傷。IgG1同種型對照物於所測試濃度顯示僅低位準的背景殺傷。The ability of humanized and chimeric 12G6 antibodies to mediate ADCC killing of cells in vehicle CD52 was assessed. The ADCC assay was performed using the T cells isolated from healthy donor PBMCs as the target cells and performed by the chromium release assay using the method as described in Example 31 above. Figure 39 illustrates the concentration (X-axis) versus % specific lysis (Y-axis) of control IgG, chimeric 12G6 antibody, and humanized 12G6 antibody (12G6-SFD1/K11 or 12G6-SFD1/K12) used in this assay. . The results showed that the humanized 12G6 antibodies 12G6-SFD1/K11 and 12G6-SFD1/K12 media were comparable to the 12G6 chimeric antibodies for ADCC killing. The IgGl isotype control showed only low level background killing at the concentrations tested.

實例36:嵌合及人類化12G6單株抗體CDC活性之評估Example 36: Evaluation of chimeric and humanized 12G6 monoclonal antibody CDC activity

評估人類化及嵌合12G6抗體於媒介CD52表現細胞的補體依賴細胞毒性(CDC)之能力。CDC試驗係如在上文實例32所敘述,使用自健康捐贈者PBMCs分離的T細胞做為標的細胞並藉由鉻釋出試驗而執行。第40圖說明用於此試驗中對照IgG、嵌合12G6抗體、及人類化12G6抗體(12G6-SFD1/K11及12G6-SFD1/K12)的濃度(X軸)相對於%特定裂解(Y軸)。結果顯示嵌合12G6抗體媒介較人類化12G6抗體(12G6-SFD1/K11及12G6-SFD1/K12)為相當的裂解。對照IgGl同種型抗體於所測試濃度顯示僅低位準的背景殺傷。The ability of humanized and chimeric 12G6 antibodies to express complement-dependent cytotoxicity (CDC) of cells in vehicle CD52 was assessed. The CDC assay was performed as described in Example 32 above, using T cells isolated from healthy donor PBMCs as target cells and performed by a chromium release assay. Figure 40 illustrates the concentration (X-axis) versus % specific lysis (Y-axis) of control IgG, chimeric 12G6 antibody, and humanized 12G6 antibody (12G6-SFD1/K11 and 12G6-SFD1/K12) used in this assay. . The results showed that the chimeric 12G6 antibody vector was comparable to the humanized 12G6 antibody (12G6-SFD1/K11 and 12G6-SFD1/K12). Control IgGl isotype antibodies showed only low level background killing at the concentrations tested.

實例37:嵌合及人類化9D9單株抗體ADCC活性之評估Example 37: Evaluation of ADCC activity of chimeric and humanized 9D9 monoclonal antibodies

評估人類化及嵌合9D9抗體於媒介CD52表現細胞的ADCC殺傷之能力。ADCC試驗係如在上文實例31所敘述,使用自健康捐贈者PBMCs分離的T細胞做為標的細胞並藉由鉻釋出試驗而執行。第41圖說明用於此試驗中對照IgG、嵌合9D9抗體、及人類化9D9抗體(9D9-H10/K13、9D9-H11/K13、9D9-H16/K13、及9D9-H18/K13)的濃度(X軸)相對於%特定裂解(Y軸)。結果顯示嵌合及人類化9D9抗體(9D9-H10/K13為例外)媒介相當的ADCC殺傷。IgGl同種型對照物於所測試濃度顯示僅低位準的背景殺傷。The ability of humanized and chimeric 9D9 antibodies to mediate ADCC killing of cells in vehicle CD52 was assessed. The ADCC assay was performed as described in Example 31 above, using T cells isolated from healthy donor PBMCs as target cells and performed by a chromium release assay. Figure 41 illustrates the concentrations of control IgG, chimeric 9D9 antibody, and humanized 9D9 antibody (9D9-H10/K13, 9D9-H11/K13, 9D9-H16/K13, and 9D9-H18/K13) used in this assay. (X-axis) Relative to % specific lysis (Y-axis). The results showed that chimeric and humanized 9D9 antibodies (with the exception of 9D9-H10/K13) media comparable ADCC killing. The IgGl isotype control showed only low level background killing at the concentrations tested.

實例38:嵌合及人類化9D9單株抗體CDC活性之評估Example 38: Evaluation of chimeric and humanized 9D9 monoclonal antibody CDC activity

評估人類化及嵌合9D9抗體於媒介CD52表現細胞的補體依賴細胞毒性(CDC)之能力。CDC試驗係如在上文實例32所敘述,使用自健康捐贈者PBMCs分離的T細胞做為標的細胞並藉由鉻釋出試驗而執行。第42圖說明用於此試驗中對照IgG、嵌合9D9抗體、及人類化9D9抗體(9D9-H10/K13、9D9-H11/K13、9D9-H16/K13、及9D9-H18/K13)的濃度(X軸)相對於%特定裂解(Y軸)。結果顯示嵌合9D9抗體媒介較人類化9D9抗體(9D9-H10/K13為例外)為相當的裂解。對照IgG1同種型抗體於所測試濃度顯示僅低位準的背景殺傷。The ability of humanized and chimeric 9D9 antibodies to express complement-dependent cytotoxicity (CDC) of cells in vehicle CD52 was assessed. The CDC assay was performed as described in Example 32 above, using T cells isolated from healthy donor PBMCs as target cells and performed by a chromium release assay. Figure 42 illustrates the concentrations of control IgG, chimeric 9D9 antibody, and humanized 9D9 antibody (9D9-H10/K13, 9D9-H11/K13, 9D9-H16/K13, and 9D9-H18/K13) used in this assay. (X-axis) Relative to % specific lysis (Y-axis). The results show that the chimeric 9D9 antibody vector is comparable to the humanized 9D9 antibody (with the exception of 9D9-H10/K13). Control IgGl isotype antibodies showed only low level background killing at the concentrations tested.

實例39:Campath-1H 及人類化抗-CD52抗體於初生T細胞的ADCC活性之評估 Example 39: Campath-1H And evaluation of ADCC activity of humanized anti-CD52 antibody in primary T cells

評估Campath-1H及人類化抗-CD52抗體於媒介CD52表現細胞的ADCC殺傷之能力。ADCC試驗係如在上文實例31所敘述,使用自健康捐贈者PBMCs分離的T細胞做為標的細胞並藉由鉻釋出試驗而執行。第43圖說明用於此試驗中對照IgG、Campath-1H、及人類化2C3-SFD1/K12、9D9-H16/K13、9D9-H18/K13、12G6-SFD1/K11、及12G6-SFD1/K12抗體的濃度(X軸)相對於%特定裂解(Y軸)。結果顯示上述人類化2C3、9D9及12G6抗體在超過10奈克/毫升的濃度媒介與Campath-1H相當的ADCC殺傷。IgG1同種型對照於所測試濃度顯示僅低位準的背景殺傷。Evaluation of Campath-1H And the human anti-CD52 antibody expresses the ADCC killing ability of the cells in the medium CD52. The ADCC assay was performed as described in Example 31 above, using T cells isolated from healthy donor PBMCs as target cells and performed by a chromium release assay. Figure 43 illustrates the control IgG, Campath-1H used in this assay. And humanized 2C3-SFD1/K12, 9D9-H16/K13, 9D9-H18/K13, 12G6-SFD1/K11, and 12G6-SFD1/K12 antibody concentrations (X-axis) versus % specific lysis (Y-axis) . The results show that the above humanized 2C3, 9D9 and 12G6 antibodies are in a concentration medium over 10 Ng/ml with Campath-1H. Quite ADCC kills. The IgGl isotype control showed only low level background killing at the concentrations tested.

實例40:Campath-1H 及人類化抗-CD52抗體於初生T細胞的CDC活性之評估 Example 40: Campath-1H And evaluation of CDC activity of humanized anti-CD52 antibody in primary T cells

評估Campath-1H及人類化抗-CD52抗體於媒介CD52表現細胞的補體依賴細胞毒性(CDC)之能力。CDC試驗係如在上文實例32所敘述,使用自健康捐贈者PBMCs分離的T細胞做為標的細胞並藉由鉻釋出試驗而執行。第44圖說明用於此試驗中對照IgG、Campath-1H、及人類化2C3-SFD1/K12、9D9-H16/K13、9D9-H18/K13、12G6-SFD1/K11、及12G6-SFD1/K12抗體的濃度(X軸)相對於%特定裂解(Y軸)。結果顯示人類化2C3及12G6抗體媒介與Campath-1H相當的CDC殺傷,然而人類化9D9抗體證實顯著減少的CDC活性,類似於其相對應嵌合抗體。IgG1同種型對照物於所測試濃度顯示僅低位準的背景殺傷。Evaluation of Campath-1H And the ability of the humanized anti-CD52 antibody to express the complement dependent cytotoxicity (CDC) of the cells in the vehicle CD52. The CDC assay was performed as described in Example 32 above, using T cells isolated from healthy donor PBMCs as target cells and performed by a chromium release assay. Figure 44 illustrates the control IgG, Campath-1H used in this assay. And humanized 2C3-SFD1/K12, 9D9-H16/K13, 9D9-H18/K13, 12G6-SFD1/K11, and 12G6-SFD1/K12 antibody concentrations (X-axis) versus % specific lysis (Y-axis) . The results show that humanized 2C3 and 12G6 antibody vectors and Campath-1H A comparable CDC kill, however, the humanized 9D9 antibody demonstrated significantly reduced CDC activity, similar to its corresponding chimeric antibody. The IgGl isotype control showed only low level background killing at the concentrations tested.

實例41:包含抗-Campath-1H 中和抗體的血清樣品阻擋人類化2C3、12G6、及9D9抗-CDS2抗體活性的中和能力之評估 Example 41: Containing anti-Campath-1H Neutralizing ability of neutralizing antibody serum samples to block the activity of humanized 2C3, 12G6, and 9D9 anti-CDS2 antibodies

為評估在抗Campath-1H的中和抗體存在下人類化抗體結合至CD52表現細胞的能力,將抗-CD52抗體(Campath-1H、2C3-SFD1/K12、9D9-H16/K13及12G6-SFD1/K12)與包含抗-Campath-1H抗體反應性的人類血清反應,並評估其至CD52表現Raji細胞之結合。自加入CAMMS223研究(The CAMMS223 Trial Investigators,"Alemtuzumab vs. interferon Beta-1a in early multiple sclerosis,"N Engl J Med 359:1786-1801(2008))的復發型多發性硬化症病人所得到的血清樣品被用於此試驗中。在大多數病人中,Campath-1H抗體的重複投藥造成抗-Campath-1H抗體反應的產生。在大多數病人中,抗-Campath-1H抗體滴度於第12個月為非常低的,並在第二循環的Campath-1H投藥時顯著增加,在第13個月於血清中產生高滴度抗-Campath-1H反應。使用得自五個不同MS病人(MS-1至MS-5)(其已在CAMMS223步驟流程下使用Campath-1H治療)第12個月及第13個月的血清樣品進行抗-CD52抗體中和試驗,在得自已使用Campath-1H治療的病人的一範圍內的血清稀釋液的存在或不存在下,FITC-共軛抗-CD52抗體Campath-1H、2C3-SFD1/K12、12G6-SFD1/K12、及9D9-H16/K13(用於實例30及顯示會結合至CD52表現細胞)被用於染色表現人類CD52的Raji細胞。簡言之,將MS病人血清樣品(第12個月及第13個月)製成6倍連續稀釋,並使用10微克/毫升的FITC-共軛抗-CD52抗體(Campath-1H、2C3-SFD1/K12、12G6-SFD1/K12、及9D9-H16/K13)於37℃培養1小時。將Raji細胞以包含HBSS、5% FBS、及0.1%疊氮化物的染色緩衝液的潤洗,及接著以每孔1 x 105細胞沉積至圓底96孔培養盤。使用10微克/毫升的人類IgG Fc片段在染色緩衝液中於冰上阻擋細胞30分鐘,接著將細胞以染色緩衝液洗並再懸浮於100微升的上述抗體-血清混合物。在於冰上30分鐘之後,沖洗細胞及以BD Cytofix固定並使用FACSCalibur系統(Becton Dickinson)分析經FITC-標記抗體塗佈的細胞,之後使用FlowJo version 7.2軟體(Tree Star,Inc,Oregon,USA)分析數據,在抗-Campath-1H中和抗體存在下,血清中FITC-共軛抗-CD52抗體的結合係由流式細胞計數法評估並相對於對照組的%結合,其為抑制的量度並以X 100計算(MFI具血清/MFI對照組(無血清))。得自提供者(MS-1)其中一個的代表性數據示於第45圖,X軸表示血清稀釋因子及Y軸表示%對照結合做為抗體中和活性之量度。數據清楚證實第12個月血清樣品於Campath-1H或其他抗-CD52抗體不具任何抑制作用,其表示血清中為低或不存在抗-Campath-1H阻斷抗體。第13個月血清樣品即使在1:1000稀釋的血清中仍媒介Campath-1H結合的完全抑制,但即使在所測試最高濃度(1:24稀釋)仍不會媒介2C3、12G6、及9D9人類化抗-CD52抗體的抑制。五個病人中的兩個發展出>1:1000的抗-Campath-1H中和抗體滴度,然而其他三個病人具約1:100 Campath-1H中和抗體滴度。即使這些病人中的兩個於第13個月血清具相當高的、>1:1000的抗-Campath-1H中和抗體滴度,這些血清不會抑制人類化2C3-SFD1/K12、12G6-SFD1/K12、及9D9-H16/K13抗體的結合,其表示在使用Campath-1H治療的病人中抗-Campath-1H抗體反應性不會阻擋這些人類化抗體至存在於細胞的CD52之結合。For evaluation in anti-Campath-1H The ability of humanized antibodies to bind to CD52 expressing cells in the presence of neutralizing antibodies, anti-CD52 antibody (Campath-1H) , 2C3-SFD1/K12, 9D9-H16/K13 and 12G6-SFD1/K12) and contain anti-Campath-1H Antibody-reactive human serum reacts and assesses its binding to CD52-expressing Raji cells. Serum samples obtained from patients with relapsing multiple sclerosis who were enrolled in the CAMMS223 study (The CAMMS223 Trial Investigators, "Alemtuzumab vs. interferon Beta-1a in early multiple sclerosis," N Engl J Med 359: 1786-1801 (2008)) Used in this test. In most patients, Campath-1H Repeated administration of antibodies results in anti-Campath-1H Production of antibody responses. In most patients, anti-Campath-1H Antibody titers were very low at 12 months and in the second cycle of Campath-1H Significantly increased when administered, producing high titer anti-Campath-1H in serum at 13th month reaction. Use from five different MS patients (MS-1 to MS-5) (which has been used with Campath-1H in the CAMMS 223 step procedure) Serum samples from the 12th and 13th months of the anti-CD52 antibody neutralization test, obtained from the used Campath-1H Treatment of patients with a range of serum dilutions in the presence or absence of FITC-conjugated anti-CD52 antibody Campath-1H 2C3-SFD1/K12, 12G6-SFD1/K12, and 9D9-H16/K13 (for Example 30 and showing binding to CD52 expressing cells) were used to stain Raji cells expressing human CD52. Briefly, MS patient serum samples (12th and 13th months) were serially diluted 6-fold and 10 μg/ml FITC-conjugated anti-CD52 antibody (Campath-1H) was used. 2C3-SFD1/K12, 12G6-SFD1/K12, and 9D9-H16/K13) were incubated at 37 ° C for 1 hour. The Raji cells were rinsed comprising HBSS, 5% FBS, staining buffer and 0.1% azide, followed by per well and 1 x 10 5 cells are deposited into round bottom 96 well plate. The cells were blocked on ice for 30 minutes in staining buffer using a 10 μg/ml human IgG Fc fragment, then the cells were washed with staining buffer and resuspended in 100 μl of the above antibody-serum mixture. After 30 minutes on ice, the cells were washed and fixed with BD Cytofix and analyzed with FITC-labeled antibody-coated cells using a FACSCalibur system (Becton Dickinson), followed by analysis using FlowJo version 7.2 software (Tree Star, Inc, Oregon, USA). Data, in anti-Campath-1H In the presence of neutralizing antibodies, the binding line of FITC-conjugated anti-CD52 antibody in serum was assessed by flow cytometry and bound to % of the control, which is a measure of inhibition and calculated as X 100 (MFI with serum/ MFI control group (no serum)). Representative data from one of the providers (MS-1) is shown in Figure 45, with the X-axis representing the serum dilution factor and the Y-axis representing % control binding as a measure of antibody neutralizing activity. Data clearly confirm the 12th month serum sample in Campath-1H Or other anti-CD52 antibodies do not have any inhibitory effect, which means low or no anti-Campath-1H in serum. Block antibodies. Serum samples from the 13th month, even in the 1:1000 dilution of serum, still mediate Campath-1H Complete inhibition of binding, but did not mediate inhibition of 2C3, 12G6, and 9D9 humanized anti-CD52 antibodies even at the highest concentration tested (1:24 dilution). Two of the five patients developed >1:1000 anti-Campath-1H Neutralizing antibody titers, however the other three patients have approximately 1:100 Campath-1H Neutralize antibody titers. Even though two of these patients had a fairly high serum of >1:1000 anti-Campath-1H at 13 months Neutralizing antibody titers, these sera do not inhibit the binding of humanized 2C3-SFD1/K12, 12G6-SFD1/K12, and 9D9-H16/K13 antibodies, which is indicated by the use of Campath-1H Anti-Campath-1H in treated patients Antibody reactivity does not block the binding of these humanized antibodies to CD52 present in the cells.

實例42:huCD52基因轉殖老鼠中抗-CD52抗體消耗及再增殖之分析(4B10-H1/K1)Example 42: Analysis of anti-CD52 antibody consumption and repopulation in huCD52 transgenic mice (4B10-H1/K1)

於huCD52基因轉殖老鼠中檢視Campath-1H及人類化抗-CD52抗體(4B10-H1/K1)於不同給藥位準下的消耗活性。將老鼠靜脈內注射0.1、0.5、1.0或5.0毫克/公斤的每一抗體,給藥後兩小時,收集血清以檢查循環細胞介素位準。給藥後三天,殺死老鼠,及從每一隻老鼠(N=5)收集血液及脾臟以使用流式細胞計數法分析來測定細胞消耗位準。評估樣品以測定存在於huCD52基因轉殖老鼠的循環週邊血液或脾臟的總T輔助細胞(CD4+)、細胞毒性T細胞(CD8+)、B細胞(B220+)及骨髓樣的細胞子族群之相對數目。此外,執行T及B細胞子組分析以測定總消耗作用。保持老鼠(N=5)子組活著以監控再增殖動力。在T細胞部份消耗最大,且CD4+T細胞消耗最多,接著為CD8+T細胞、B細胞、NK細胞、及其他骨髓樣的細胞。在CD4+T細胞部份內,自然(nave)CD4+T細胞消耗最多,接著為CD4+中樞記憶性(CM)、CD4+效應記憶性(EM)、及CD4+調節T細胞(Treg)。類似形式亦於CD8+T細胞(Nave>CM>EM)觀察到,相反地,成熟B細胞較不成熟B細胞消耗程度為大。經Campath-1H治療之老鼠與經4B10-H1/K1治療之老鼠的比較證實於每一個所測試的劑量血液及脾臟兩者中細胞皆具類似型式。Examination of Campath-1H in huCD52 transgenic mice And the humanized anti-CD52 antibody (4B10-H1/K1) was depleted at different administration levels. The rats were intravenously injected with 0.1, 0.5, 1.0 or 5.0 mg/kg of each antibody, and two hours after the administration, serum was collected to examine the circulating cytokine level. Three days after the administration, the mice were sacrificed, and blood and spleens were collected from each mouse (N=5) to determine the level of cell consumption using flow cytometry analysis. Samples were evaluated to determine the relative number of total T helper cells (CD4+), cytotoxic T cells (CD8+), B cells (B220+), and myeloid cell subpopulations present in the circulating peripheral blood or spleen of huCD52 gene-transferred mice. In addition, T and B cell subgroup analyses were performed to determine total depletion. The mouse (N=5) subgroup was kept alive to monitor repopulation dynamics. The T cell fraction is most consumed, and CD4+ T cells are most consumed, followed by CD8+ T cells, B cells, NK cells, and other bone marrow-like cells. Within the CD4+ T cell part, nature (na Ve) CD4+ T cells are most consumed, followed by CD4+ central memory (CM), CD4+ effector memory (EM), and CD4+ regulatory T cells (Treg). A similar form is also found in CD8+ T cells (Na Ve>CM>EM) Observed, on the contrary, mature B cells consumed more than immature B cells. By Campath-1H Comparison of treated mice with 4B10-H1/K1 treated mice confirmed that the cells in each of the tested doses of blood and spleen had similar patterns.

血清細胞介素分析證實對TNFα、IL-6及MCP-1劑量相依增加,相較於未經治療之老鼠,在0.5及0.1毫克/公斤劑量下這些細胞介素的循環位準也維持升高。在三個最高劑量下在經Campath-1H治療的群組中觀察到IL-10也些微增加,但對於經人類化4B10-H1/K1治療群組僅對最高劑量觀察到些微增加。在循環IL-12或IFNg(未示出)位準沒有注意到任何顯著增加。Serum interleukin analysis confirmed a dose-dependent increase in TNFα, IL-6, and MCP-1, and the circulating levels of these interleukins were also elevated at 0.5 and 0.1 mg/kg compared to untreated mice. . At the three highest doses in the Campath-1H A slight increase in IL-10 was also observed in the treated groups, but only a slight increase was observed for the highest dose at the humanized 4B10-H1/K1 treatment group. No significant increase was noted at the circulating IL-12 or IFNg (not shown) levels.

給藥後50-60天,除了1.0毫克/公斤組,在所有經Campath-1H給藥組中淋巴細胞位準回到未經治療老鼠的位準。在1.0毫克/公斤組,給藥後80天淋巴細胞回到正常位準。類似再增殖動力亦於經人類化4B10-H1/K1抗體治療之老鼠觀察到,在所有經4B10-H1/K1治療組在給藥後50天,除了0.5毫克/公斤位準,淋巴細胞回到對照組位準。於0.5毫克/公斤組,循環淋巴細胞位準經過監控期間的過程維持減少。針對血液中再增殖而監控總淋巴細胞。50-60 days after dosing, except for the 1.0 mg/kg group, at all via Campath-1H The level of lymphocytes in the drug-administered group returned to the level of untreated mice. In the 1.0 mg/kg group, lymphocytes returned to normal levels 80 days after dosing. Similar re-proliferation motility was also observed in mice treated with the humanized 4B10-H1/K1 antibody, and all lymphocytes returned to the 4B10-H1/K1 treatment group 50 days after administration, except for the 0.5 mg/kg level. The control group was level. At the 0.5 mg/kg group, the process of circulating lymphocyte levels during maintenance was reduced. Total lymphocytes are monitored for repopulation in the blood.

第46A-46E圖顯示在使用Campath-1H(「Campath」)及人類化4B10-H1/K1(「4B10」)抗體投藥後72小時血液中CD4+ T細胞、CD8+ T細胞及B220+ B細胞的含量。第47A-47E圖顯示在使用Campath-1H(「Campath」)及人類化4B10-H1/K1(「4B10」)抗體投藥後72小時脾臟中CD4+ T細胞、CD8+ T細胞及B220+ B細胞的含量。第48A-48E圖顯示在使用Campath-1H(「Campath」)及人類化4B10-H1/K1(「4B10」)抗體投藥後2小時循環細胞介素位準。第49A-49B圖顯示在使用Campath-1H(「Campath」)及人類化4B10-H1/K1(「4B10」)抗體投藥後循環淋巴細胞隨時間的再增殖。Figure 46A-46E shows the use of Campath-1H ("Campath") and the content of CD4+ T cells, CD8+ T cells and B220+ B cells in the blood 72 hours after administration of the humanized 4B10-H1/K1 ("4B10") antibody. Figure 47A-47E shows the use of Campath-1H ("Campath") and the content of CD4+ T cells, CD8+ T cells and B220+ B cells in the spleen 72 hours after administration of the humanized 4B10-H1/K1 ("4B10") antibody. Figure 48A-48E shows the use of Campath-1H ("Campath") and humanized 4B10-H1/K1 ("4B10") antibody circulating the cytokine level 2 hours after administration. Figure 49A-49B shows the use of Campath-1H ("Campath") and humanized 4B10-H1/K1 ("4B10") antibody repopulated with circulating lymphocytes over time.

實例43:huCD52基因轉殖老鼠中抗-CD52抗體的消耗及再增殖之分析(7F11-SFD1/K2及7F11-SFD2/K2)Example 43: Analysis of consumption and repopulation of anti-CD52 antibodies in huCD52 transgenic mice (7F11-SFD1/K2 and 7F11-SFD2/K2)

於huCD52基因轉殖老鼠中檢視人類化抗體(7F11-SFD1/K2及7F11-SFD2/K2)於不同劑量位準的的消耗活性。將老鼠靜脈內注射0.1、0.5、1.0或5.0毫克/公斤的每一抗體,給藥後兩小時,收集血清以檢查循環細胞介素位準。給藥後三天,殺死老鼠,及從每一隻老鼠(N=5)收集血液及脾臟以使用流式細胞計數法分析來測定細胞消耗位準。評估樣品以測定存在於huCD52基因轉殖老鼠的循環週邊血液或脾臟的總T輔助細胞(CD4+)、細胞毒性T細胞(CD8+)、B細胞(B220+)及骨髓樣的細胞子族群之相對數目。此外,執行T及B細胞子組分析以測定總消耗作用,保持老鼠(N=5)子組活著以監控再增殖動力。以所有劑量投藥每一人類化7F11抗體(7F11-SFD1/K2及7F11-SFD2/K2)產生血液中顯著數目的T細胞及B細胞的消耗,這些數據亦證實各種T及B細胞子組依據所使用抗體劑量不同程度而被消耗。自然T細胞(CD4與CD8兩者)證實為最大消耗且其他細胞族群(包含記憶性及T調節細胞)較少程度地消耗。在B細胞部份,成熟B細胞較不成熟B細胞消耗更快速。在脾臟中,觀察到隨著於5及1毫克/公斤劑量位準所觀察到的淋巴細胞的顯著消耗之劑量相依消耗。類似於在血液的情況,自然T細胞較記憶性細胞消耗更快速。使用人類化7F11細胞株(7F11-SFD1/K2及7F11-SFD2/K2)的每一個,B細胞較T細胞消耗程度較少。在任何注射劑量於血液或脾臟中對NK細胞或嗜中性球沒有觀察到任何消耗。血清細胞介素分析證實對TNF及IL-6兩者的劑量相依,相較於未經治療老鼠,在0.5及0.1毫克/公斤劑量這些細胞介素的位準也維持升高。亦觀察到於循環MCP-1位準的劑量相依增加。The humanized antibodies (7F11-SFD1/K2 and 7F11-SFD2/K2) were examined for their depletion activity at different dose levels in huCD52 transgenic mice. The rats were intravenously injected with 0.1, 0.5, 1.0 or 5.0 mg/kg of each antibody, and two hours after the administration, serum was collected to examine the circulating cytokine level. Three days after the administration, the mice were sacrificed, and blood and spleens were collected from each mouse (N=5) to determine the level of cell consumption using flow cytometry analysis. Samples were evaluated to determine the relative number of total T helper cells (CD4+), cytotoxic T cells (CD8+), B cells (B220+), and myeloid cell subpopulations present in the circulating peripheral blood or spleen of huCD52 gene-transferred mice. In addition, T and B cell subgroup analyses were performed to determine total depletion and mice (N=5) subgroups were kept alive to monitor repopulation motility. Administration of each humanized 7F11 antibody (7F11-SFD1/K2 and 7F11-SFD2/K2) at all doses produced significant amounts of T cells and B cells in the blood. These data also confirmed various T and B cell subgroups. The antibody dose is consumed to varying degrees. Natural T cells (both CD4 and CD8) were confirmed to be the most consumed and other cell populations (including memory and T regulatory cells) were consumed to a lesser extent. In the B cell fraction, mature B cells consume more rapidly than immature B cells. In the spleen, a dose-dependent consumption of significant consumption of lymphocytes observed with the 5 and 1 mg/kg dose levels was observed. Similar to the case of blood, natural T cells consume more quickly than memory cells. Using each of the humanized 7F11 cell lines (7F11-SFD1/K2 and 7F11-SFD2/K2), B cells were less consumed than T cells. No consumption was observed for NK cells or neutrophils in any of the injected doses in the blood or spleen. Serum interleukin analysis confirmed dose-dependent dependence on both TNF and IL-6, and the levels of these interleukins were also elevated at 0.5 and 0.1 mg/kg compared to untreated mice. A dose-dependent increase in circulating MCP-1 levels was also observed.

給藥後30天,在0.5及0.1毫克/公斤給藥組中淋巴細胞位準回到未經治療老鼠的位準。在1.0及5.0毫克/公斤組,針對細胞株7F11-SFD1/K2,分別給藥50及80天淋巴細胞回到正常位準,及對細胞株7F11-SFD2/K2的1.0及5.0毫克/公斤組為給藥後80天。針對血液中再增殖而監控總淋巴細胞。At 30 days after administration, the lymphocyte level returned to the level of untreated mice in the 0.5 and 0.1 mg/kg administration groups. In the 1.0 and 5.0 mg/kg groups, the cell line 7F11-SFD1/K2 was administered 50 and 80 days, respectively, and the lymphocytes returned to the normal level, and the cell line 7F11-SFD2/K2 was 1.0 and 5.0 mg/kg. For 80 days after administration. Total lymphocytes are monitored for repopulation in the blood.

第50A-50E圖顯示在使用人類化7F11-SFD1/K2(「7F11 SFD1」)及7F11-SFD2/K2(「7F11 SFD2」)抗體投藥後72小時血液中CD4+T細胞、CD8+T細胞及B220+B細胞的含量。第51A-51E圖顯示在使用人類化7F11-SFD1/K2(「7F11 SFD1」)及7F11-SFD2/K2(「7F11 SFD2」)抗體投藥後72小時脾臟中CD4+T細胞、CD8+T細胞及B220+B細胞的含量。第52A-52F圖顯示在使用人類化7F11-SFD1/K2(「7F11 SFD1」)及7F11-SFD2/K2(「7F11 SFD2」)抗體投藥後2小時循環細胞介素位準。第53A-53B圖顯示在使用人類化7F11-SFD1/K2(「7F11 SFD1」)及7F11-SFD2/K2(「7F11 SFD2」)抗體投藥後循環淋巴細胞隨時間的再增殖。Figure 50A-50E shows CD4+ T cells and CD8+ T cells in the blood 72 hours after administration of humanized 7F11-SFD1/K2 ("7F11 SFD1") and 7F11-SFD2/K2 ("7F11 SFD2") antibodies. The content of B220+B cells. Figure 51A-51E shows CD4+ T cells and CD8+ T cells in the spleen 72 hours after administration of humanized 7F11-SFD1/K2 ("7F11 SFD1") and 7F11-SFD2/K2 ("7F11 SFD2") antibodies. The content of B220+B cells. Figures 52A-52F show circulating interleukin levels 2 hours after administration of humanized 7F11-SFD1/K2 ("7F11 SFD1") and 7F11-SFD2/K2 ("7F11 SFD2") antibodies. Figures 53A-53B show repopulation of circulating lymphocytes over time following administration of humanized 7F11-SFD1/K2 ("7F11 SFD1") and 7F11-SFD2/K2 ("7F11 SFD2") antibodies.

實例44:CD52基因轉殖老鼠中7F11人類化抗-CD52抗體之分析(7F11-SFD1/K2及7F11-SFD2/K2)Example 44: Analysis of 7F11 humanized anti-CD52 antibody in CD52 gene transfer mice (7F11-SFD1/K2 and 7F11-SFD2/K2)

於huCD52基因轉殖老鼠中檢視嵌合7F11抗體及人類化7F11-SFD1/K2及7F11-SFD2/K2抗體與Campath-1H相較之消耗活性。將老鼠靜脈內注射1.0毫克/公斤的每一抗體。給藥後三天,殺死老鼠,及從每一隻老鼠(N=5)收集血液及脾臟以使用流式細胞計數法分析來測定細胞消耗位準。評估樣品以測定存在於huCD52基因轉殖老鼠的循環週邊血液或脾臟的總T輔助細胞(CD4+)、細胞毒性T細胞(CD8+)、B細胞(B220+)及骨髓樣的細胞子族群之相對數目。投藥Campath-1H造成血液及脾臟中顯著數目的T細胞及B細胞之消耗,雖然對嵌合及人類化7F11抗體(7F11-SFD1/K2及7F11-SFD2/K2)觀察到血液中相當位準的T細胞消耗,B細胞為較少程度地消耗。此觀察在脾臟中亦為明顯,於此注意到顯著T細胞消耗,但使用7F11抗體(7F11-SFD1/K2及7F11-SFD2/K2)僅達到中度量的B細胞消耗。Chimeric 7F11 Antibody and Humanized 7F11-SFD1/K2 and 7F11-SFD2/K2 Antibody and Campath-1H in huCD52 Gene Transgenic Rats It consumes activity compared to it. Rats were injected intravenously with 1.0 mg/kg of each antibody. Three days after the administration, the mice were sacrificed, and blood and spleens were collected from each mouse (N=5) to determine the level of cell consumption using flow cytometry analysis. Samples were evaluated to determine the relative number of total T helper cells (CD4+), cytotoxic T cells (CD8+), B cells (B220+), and myeloid cell subpopulations present in the circulating peripheral blood or spleen of huCD52 gene-transferred mice. Dosing Campath-1H A significant number of T cells and B cells are consumed in the blood and spleen, although a considerable amount of T cell consumption in the blood is observed for chimeric and humanized 7F11 antibodies (7F11-SFD1/K2 and 7F11-SFD2/K2), B cells are consumed to a lesser extent. This observation was also evident in the spleen, where significant T cell depletion was noted, but only 7F11 antibodies (7F11-SFD1/K2 and 7F11-SFD2/K2) were used to achieve only moderately measured B cell depletion.

第54A-54B圖顯示在使用Campath-1H(「Campath」)、7F11-嵌合抗體、及人類化7F11-SFD1/K2與7F11-SFD2/K2抗體投藥後72小時,血液中CD4+ T細胞、CD8+ T細胞及B220+ B細胞的含量。Figure 54A-54B shows the use of Campath-1H The content of CD4+ T cells, CD8+ T cells and B220+ B cells in the blood ("Campath"), 7F11-chimeric antibody, and humanized 7F11-SFD1/K2 and 7F11-SFD2/K2 antibodies were administered 72 hours later.

實例45:CD52基因轉殖老鼠中抗-CD52抗體之PK數據分析(7F11-SFD1/K2及7F11-SFD2/K2)Example 45: PK data analysis of anti-CD52 antibodies in CD52 transgenic mice (7F11-SFD1/K2 and 7F11-SFD2/K2)

為確保人類化製程不會變更抗體的清除速率,嵌合7F11抗-CD52抗體及人類化7F11-SFD1/K2與7F11-SFD2/K2抗-CD52抗體的藥物動力數據係於huCD52基因轉殖老鼠中測定。將老鼠靜脈內注射5毫克/公斤的抗體及在給藥後兩小時開始於各種時間點收集血液,每一個抗體的循環位準係使用抗-人類IgG ELISA評估。針對每一個人類化細胞株,在給藥後兩小時觀察的Cmax中存在些微差別。在實驗進行期間,嵌合7F11抗體及人類化7F11-SFD1/K2與7F11-SFD2/K2抗體的清除速率為彼此類似並與Campath-1H類似,其顯示人類化製程不會顯著變更抗體的藥物動力數據。To ensure that the humanization process does not alter the clearance rate of antibodies, the pharmacokinetic data for chimeric 7F11 anti-CD52 antibody and humanized 7F11-SFD1/K2 and 7F11-SFD2/K2 anti-CD52 antibodies are in huCD52 transgenic mice. Determination. Mice were injected intravenously with 5 mg/kg of antibody and blood was collected at various time points starting two hours after dosing. The circulating level of each antibody was assessed using an anti-human IgG ELISA. For each humanized cell line, there was a slight difference in the Cmax observed two hours after administration. During the course of the experiment, the clearance rates of the chimeric 7F11 antibody and the humanized 7F11-SFD1/K2 and 7F11-SFD2/K2 antibodies were similar to each other and with Campath-1H. Similarly, it shows that the humanization process does not significantly alter the pharmacokinetic data of the antibody.

第55圖顯示於給藥後血液中Campath-1H(「Campath」)、7F11-嵌合抗體及人類化7F11-SFD1/K2與7F11-SFD2/K2抗體隨時間的含量。Figure 55 shows Campath-1H in the blood after administration. ("Campath"), 7F11-chimeric antibody and humanized 7F11-SFD1/K2 and 7F11-SFD2/K2 antibody content over time.

real 例46:huCD52基因轉殖老鼠中抗-CD52抗體的消耗及再增殖之分析(2C3-SFD1/K12)Example 46: Analysis of anti-CD52 antibody consumption and repopulation in huCD52 transgenic mice (2C3-SFD1/K12)

於huCD52基因轉殖老鼠中檢視2C3-SFD1/K12細胞株於不同劑量位準的的消耗活性。將老鼠靜脈內注射0.1、0.5、1.0或5.0毫克/公斤抗體,給藥後兩小時,收集血清以潛在地檢查循環細胞介素位準。給藥後三天,殺死老鼠,及從每一隻老鼠(N=5)收集血液及脾臟,以使用流式細胞計數法分析來測定細胞消耗位準。評估樣品以測定存在於huCD52基因轉殖老鼠的循環週邊血液或脾臟的總T輔助細胞(CD4+)、細胞毒性T細胞(CD8+)、B細胞(B220+)及骨髓樣的細胞子族群之相對數目。此外,執行T及B細胞子組分析以決定總消耗作用,保持老鼠(N=5)子組活著以監控再增殖動力。在5、1、及0.5毫克/公斤劑量投藥2C3-SFD1/K12導致消耗血液中顯著數目的T細胞及B細胞。觀察到於0.1毫克/公斤劑量時血液中各種淋巴細胞消耗位準,且CD4+T細胞及B細胞較CD8+T細胞有較大消耗程度。這些數據亦證實各種T及B細胞子組依據所使用抗體劑量有不同程度的消耗。自然T細胞(CD4與CD8兩者)與其他細胞族群(包含記憶性及T調節細胞)相較被證實為最大消耗,這些細胞族群係為較少程度地消耗。在B細胞部份,成熟B細胞較不成熟B細胞消耗更快速。在脾臟,觀察到於5及1毫克/公斤劑量位準時,淋巴細胞的顯著消耗之劑量相依消耗。類似於Campath-1H,自然T細胞較記憶性細胞消耗更快速。在任何注射劑量時,於血液中對NK細胞或嗜中性球觀察到消耗,但是在脾臟中觀察到些微或沒有任何消耗。血清細胞介素分析證實對TNFα及IL-6的劑量相依增加,且5毫克/公斤劑量誘發最高位準的每一個細胞介素。在0.5及0.1毫克/公斤劑量位準針對TNFα,以及在0.1毫克/公斤劑量位準針對IL-6,觀察到可與未經治療老鼠相較的位準。亦觀察到於循環MCP-1位準的劑量相依增加。The consumption activity of 2C3-SFD1/K12 cell lines at different dose levels was examined in huCD52 transgenic mice. Mice were injected intravenously with 0.1, 0.5, 1.0 or 5.0 mg/kg of antibody, and two hours after dosing, serum was collected to potentially examine circulating cytokine levels. Three days after the administration, the mice were sacrificed, and blood and spleen were collected from each mouse (N=5) to determine the level of cell consumption using flow cytometry analysis. Samples were evaluated to determine the relative number of total T helper cells (CD4+), cytotoxic T cells (CD8+), B cells (B220+), and myeloid cell subpopulations present in the circulating peripheral blood or spleen of huCD52 gene-transferred mice. In addition, T and B cell subgroup analyses were performed to determine total depletion and mice (N=5) subgroups were kept alive to monitor repopulation motility. Administration of 2C3-SFD1/K12 at doses of 5, 1, and 0.5 mg/kg resulted in the consumption of significant numbers of T cells and B cells in the blood. The level of various lymphocyte depletion in the blood at a dose of 0.1 mg/kg was observed, and CD4+ T cells and B cells were more consumed than CD8+ T cells. These data also confirm that various T and B cell subgroups have varying degrees of consumption depending on the dose of antibody used. Natural T cells (both CD4 and CD8) have been shown to be the most consumed compared to other cell populations (including memory and T regulatory cells), which are consumed to a lesser extent. In the B cell fraction, mature B cells consume more rapidly than immature B cells. In the spleen, a significant dose of lymphocytes was consumed depending on the dose at the 5 and 1 mg/kg dose levels. Similar to Campath-1H Natural T cells consume more rapidly than memory cells. At any injected dose, consumption was observed in the blood for NK cells or neutrophils, but little or no consumption was observed in the spleen. Serum interleukin analysis confirmed a dose-dependent increase in TNFα and IL-6, and a dose of 5 mg/kg induced the highest level of each interleukin. At the dose levels of 0.5 and 0.1 mg/kg for TNFα, and at the 0.1 mg/kg dose level for IL-6, levels comparable to untreated mice were observed. A dose-dependent increase in circulating MCP-1 levels was also observed.

給藥後30天,在0.1及0.5毫克/公斤組中淋巴細胞位準回到未經治療老鼠的位準。在1.0及5.0毫克/公斤組,給藥後80天淋巴細胞回到正常位準。針對血液中再增殖而監控總淋巴細胞。At 30 days after administration, lymphocyte levels returned to the level of untreated mice in the 0.1 and 0.5 mg/kg groups. In the 1.0 and 5.0 mg/kg groups, lymphocytes returned to normal levels 80 days after dosing. Total lymphocytes are monitored for repopulation in the blood.

第56A-56E圖顯示在使用2C3-SFD1/K12抗體投藥後72小時血液中CD4+T細胞、CD8+T細胞及B220+B細胞的含量。第57A-57E圖顯示在使用2C3-SFD1/K12抗體投藥後72小時脾臟中CD4+T細胞、CD8+T細胞及B220+B細胞的含量。第58A-58F圖顯示在使用2C3-SFD1/K12抗體投藥後2小時循環細胞介素位準。第59圖顯示在使用2C3-SFD1/K12抗體投藥後循環淋巴細胞隨時間的再增殖。Figures 56A-56E show the levels of CD4+ T cells, CD8+ T cells, and B220+ B cells in the blood 72 hours after administration with the 2C3-SFD1/K12 antibody. Figures 57A-57E show the levels of CD4+ T cells, CD8+ T cells, and B220+ B cells in the spleen 72 hours after administration with the 2C3-SFD1/K12 antibody. Figures 58A-58F show circulating interleukin levels 2 hours after administration with the 2C3-SFD1/K12 antibody. Figure 59 shows repopulation of circulating lymphocytes over time following administration with the 2C3-SFD1/K12 antibody.

實例47:huCD52基因轉殖老鼠中抗-CD52抗體的消耗及再增殖之分析(12G6-SFD1/K11)Example 47: Analysis of consumption and repopulation of anti-CD52 antibody in huCD52 transgenic mice (12G6-SFD1/K11)

於huCD52基因轉殖老鼠中檢視12G6-SFD1/K11細胞株於不同劑量位準的消耗活性。將老鼠靜脈內注射0.1、0.5、1.0或5.0毫克/公斤抗體,給藥後兩小時,收集血清以潛在地檢查循環細胞介素位準。給藥後三天,殺死老鼠,及從每一隻老鼠(N=5)收集血液及脾臟,以使用流式細胞計數法分析測定細胞消耗位準。評估樣品以測定存在於huCD52基因轉殖老鼠的循環週邊血液或脾臟的總T輔助細胞(CD4+)、細胞毒性T細胞(CD8+)、B細胞(B220+)及骨髓樣的細胞子族群之相對數目。此外,執行T及B細胞子組分析以測定總消耗作用,保持老鼠(N=5)子組活著以監控再增殖動力。在5、1、及0.5毫克/公斤劑量投藥12G6-SFD1/K11導致消耗血液中顯著數目的T細胞及B細胞,於0.1毫克/公斤劑量時,觀察到血液中各種淋巴細胞消耗位準,且CD4+T細胞及B細胞較CD8+T細胞有較大消耗程度。這些數據亦證實各種T及B細胞子組依據所使用的抗體劑量不同程度地消耗。自然T細胞(CD4與CD8兩者)與其他細胞族群(包含記憶性及T調節細胞)相較被證實為最大消耗,這些細胞族群係為較少程度地消耗。在B細胞部份,成熟B細胞較不成熟B細胞消耗更快速。在脾臟,觀察到在5及1毫克/公斤劑量位準時淋巴細胞的顯著消耗之劑量相依消耗。類似於Campath-1H,自然T細胞較記憶性細胞消耗更快速。在任何注射劑量,於血液中對NK細胞或嗜中性球觀察到消耗,但是在脾臟中觀察到些微或沒有任何消耗。血清細胞介素分析證實對TNFα及IL-6兩者的劑量相依增加,且5毫克/公斤劑量誘發最高位準的每一個細胞介素。在0.5及0.1毫克/公斤劑量位準針對TNFα,以及在0.1毫克/公斤劑量位準針對IL-6,觀察到可與未經治療老鼠相較的位準。亦觀察到於循環MCP-1位準的劑量相依增加。The depletion activity of 12G6-SFD1/K11 cell lines at different dose levels was examined in huCD52 transgenic mice. Mice were injected intravenously with 0.1, 0.5, 1.0 or 5.0 mg/kg of antibody, and two hours after dosing, serum was collected to potentially examine circulating cytokine levels. Three days after the administration, the mice were sacrificed, and blood and spleen were collected from each mouse (N=5) to determine the level of cell consumption by flow cytometry analysis. Samples were evaluated to determine the relative number of total T helper cells (CD4+), cytotoxic T cells (CD8+), B cells (B220+), and myeloid cell subpopulations present in the circulating peripheral blood or spleen of huCD52 gene-transferred mice. In addition, T and B cell subgroup analyses were performed to determine total depletion and mice (N=5) subgroups were kept alive to monitor repopulation motility. Administration of 12G6-SFD1/K11 at doses of 5, 1, and 0.5 mg/kg resulted in the consumption of significant numbers of T cells and B cells in the blood, and at the dose of 0.1 mg/kg, various levels of lymphocyte depletion were observed in the blood, and CD4+ T cells and B cells have a greater degree of consumption than CD8+ T cells. These data also confirm that various T and B cell subgroups are consumed to varying degrees depending on the dose of antibody used. Natural T cells (both CD4 and CD8) have been shown to be the most consumed compared to other cell populations (including memory and T regulatory cells), which are consumed to a lesser extent. In the B cell fraction, mature B cells consume more rapidly than immature B cells. In the spleen, a dose-dependent consumption of significant consumption of lymphocytes at the 5 and 1 mg/kg dose levels was observed. Similar to Campath-1H Natural T cells consume more rapidly than memory cells. At any injected dose, consumption was observed in the blood for NK cells or neutrophils, but little or no consumption was observed in the spleen. Serum interleukin analysis confirmed a dose-dependent increase in both TNFα and IL-6, and a dose of 5 mg/kg induced the highest level of each interleukin. At the dose levels of 0.5 and 0.1 mg/kg for TNFα, and at the 0.1 mg/kg dose level for IL-6, levels comparable to untreated mice were observed. A dose-dependent increase in circulating MCP-1 levels was also observed.

給藥後30天,淋巴細胞位準回到未經治療老鼠的位準。在1.0及5.0毫克/公斤組,給藥後80天淋巴細胞回到正常位準。針對血液中再增殖而監控總淋巴細胞。At 30 days after administration, lymphocyte levels returned to the level of untreated mice. In the 1.0 and 5.0 mg/kg groups, lymphocytes returned to normal levels 80 days after dosing. Total lymphocytes are monitored for repopulation in the blood.

第60A-60E圖顯示在使用12G6-SFD1/K11抗體投藥後72小時血液中CD4+T細胞、CD8+T細胞及B220+B細胞的含量。第61A-61E圖顯示在使用12G6-SFD1/K11抗體投藥後72小時脾臟中CD4+T細胞、CD8+T細胞及B220+B細胞的含量。第62A-62F圖顯示在使用12G6-SFD1/K11(「12G6hu」)抗體投藥後2小時循環細胞介素位準。第63圖顯示在使用12G6-SFD1/K11抗體投藥後循環淋巴細胞隨時間的再增殖。Figures 60A-60E show the levels of CD4+ T cells, CD8+ T cells, and B220+ B cells in the blood 72 hours after administration with the 12G6-SFD1/K11 antibody. Panels 61A-61E show the levels of CD4+ T cells, CD8+ T cells, and B220+ B cells in the spleen 72 hours after administration with the 12G6-SFD1/K11 antibody. Panels 62A-62F show circulating interleukin levels 2 hours after administration with 12G6-SFD1/K11 ("12G6hu") antibody. Figure 63 shows repopulation of circulating lymphocytes over time following administration with 12G6-SFD1/K11 antibody.

實例48:CD52基因轉殖老鼠中抗-CD52抗體之PK數據分析(2C3-SFD1/K12、12G6-SFD1/K11及9D9-H10/K12)Example 48: PK data analysis of anti-CD52 antibodies in CD52 transgenic mice (2C3-SFD1/K12, 12G6-SFD1/K11 and 9D9-H10/K12)

抗-CD52抗體的藥物動力數據係於huCD52基因轉殖老鼠中測定,此實驗比較抗體的人類化及嵌合形式,以確保人類化製程不會變更抗體的清除速率。所述比較包含嵌合2C3、12G6、及9D9抗體及人類化2C3-SFD1/K12、12G6-SFD1/K11、及9D9-H10/K12抗體。將老鼠靜脈內注射5毫克/公斤的抗體及在給藥後兩小時開始於各種時間點收集血液,每一個抗體的循環位準係使用抗-人類IgG ELISA評估。對所分析的每一個嵌合/人類化抗體對,在給藥後兩小時注意到於Cmax中有些微差別。對2C3及12G6抗體,人類化抗體(亦即,2C3-SFD1/K12及12G6-SFD1/K11)的Cmax些微較高,然而對9D9對而言嵌合抗體些微較高。在實驗進行期間抗體對的清除速率為類似的,其顯示人類化製程不會顯著變更抗體的藥物動力數據。The pharmacokinetic data for anti-CD52 antibodies were determined in huCD52 transgenic mice. This experiment compares the humanized and chimeric forms of antibodies to ensure that the humanization process does not alter the rate of antibody clearance. The comparisons included chimeric 2C3, 12G6, and 9D9 antibodies and humanized 2C3-SFD1/K12, 12G6-SFD1/K11, and 9D9-H10/K12 antibodies. Mice were injected intravenously with 5 mg/kg of antibody and blood was collected at various time points starting two hours after dosing. The circulating level of each antibody was assessed using an anti-human IgG ELISA. For each chimeric/humanized antibody pair analyzed, there was some slight difference in Cmax observed two hours after dosing. For the 2C3 and 12G6 antibodies, the Cmax of the humanized antibodies (i.e., 2C3-SFD1/K12 and 12G6-SFD1/K11) was slightly higher, whereas the chimeric antibody was slightly higher for the 9D9 pair. The rate of clearance of antibody pairs during the experiment was similar, showing that the humanization process did not significantly alter the drug motility data for the antibody.

第64A-64C圖顯示給藥後血液中2C3-嵌合、2C3-SFD1/K12,12G6-嵌合、12G6-SFD1/K11、9D9-嵌合、及9D9-H10/K12抗體隨時間的含量。Figure 64A-64C shows the levels of 2C3-chimeric, 2C3-SFD1/K12, 12G6-chimeric, 12G6-SFD1/K11, 9D9-chimeric, and 9D9-H10/K12 antibodies in the blood after administration.

實例49:huCD52基因轉殖老鼠中抗-CD52抗體的消耗及再增殖之分析(9D9-H10/K12)Example 49: Analysis of consumption and repopulation of anti-CD52 antibody in huCD52 transgenic mice (9D9-H10/K12)

於huCD52基因轉殖老鼠中檢視9D9-H10/K12細胞株於不同劑量位準的的消耗活性。將老鼠靜脈內注射0.1、0.5、1.0或5.0毫克/公斤抗體,給藥後兩小時,收集血清以潛在地檢查循環細胞介素位準。給藥後三天,殺死老鼠,及從每一隻老鼠(N=5)收集血液及脾臟,以使用流式細胞計數法分析來測定細胞消耗位準。評估樣品以測定存在於huCD52基因轉殖老鼠的循環週邊血液或脾臟的總T輔助細胞(CD4+)、細胞毒性T細胞(CD8+)、B細胞(B220+)及骨髓樣的細胞子族群之相對數目。此外,執行T及B細胞子組分析以測定總消耗作用。保持老鼠(N=5)子組活著以監控再增殖動力。在5、1、及0.5毫克/公斤劑量投藥9D9-H10/K12導致消耗血液中顯著數目的T細胞及B細胞。觀察到於0.1毫克/公斤劑量血液中僅中度的淋巴細胞消耗位準,這些數據亦證實各種T及B細胞子組依據所使用抗體劑量而不同程度地消耗。自然T細胞(CD4與CD8兩者)與其他細胞族群(包含記憶性及T調節細胞)相較被證實為最大消耗,這些細胞族群係為較少程度地消耗。在B細胞部份,成熟B細胞較不成熟B細胞消耗更快速。在脾臟,這些細胞的顯著消耗僅在5及1毫克/公斤劑量位準觀察到。類似於Campath-1H,自然T細胞較記憶性細胞消耗更快速。在任何注射劑量,於血液中對NK細胞或嗜中性球觀察到消耗,但是在脾臟中觀察到些微或沒有任何消耗。血清細胞介素分析證實對TNF或IL-6在所分析的任何劑量位準沒有顯著增加,然而,注意到在循環MCP-1位準的劑量相依增加。The consumption activity of the 9D9-H10/K12 cell line at different dose levels was examined in huCD52 transgenic mice. Mice were injected intravenously with 0.1, 0.5, 1.0 or 5.0 mg/kg of antibody, and two hours after dosing, serum was collected to potentially examine circulating cytokine levels. Three days after the administration, the mice were sacrificed, and blood and spleen were collected from each mouse (N=5) to determine the level of cell consumption using flow cytometry analysis. Samples were evaluated to determine the relative number of total T helper cells (CD4+), cytotoxic T cells (CD8+), B cells (B220+), and myeloid cell subpopulations present in the circulating peripheral blood or spleen of huCD52 gene-transferred mice. In addition, T and B cell subgroup analyses were performed to determine total depletion. The mouse (N=5) subgroup was kept alive to monitor repopulation dynamics. Administration of 9D9-H10/K12 at doses of 5, 1, and 0.5 mg/kg resulted in the consumption of significant numbers of T cells and B cells in the blood. Only moderate levels of lymphocyte depletion were observed in the 0.1 mg/kg dose of blood, and these data also confirmed that various T and B cell subgroups were consumed to varying degrees depending on the dose of antibody used. Natural T cells (both CD4 and CD8) have been shown to be the most consumed compared to other cell populations (including memory and T regulatory cells), which are consumed to a lesser extent. In the B cell fraction, mature B cells consume more rapidly than immature B cells. In the spleen, significant consumption of these cells was only observed at the 5 and 1 mg/kg dose levels. Similar to Campath-1H Natural T cells consume more rapidly than memory cells. At any injected dose, consumption was observed in the blood for NK cells or neutrophils, but little or no consumption was observed in the spleen. Serum interleukin analysis confirmed no significant increase in TNF or IL-6 at any of the dose levels analyzed, however, a dose-dependent increase in circulating MCP-1 levels was noted.

此實驗的再增殖部分係於淋巴細胞50-80%再增殖(依據劑量而定)時提早結束,淋巴細胞再增殖係基於總淋巴細胞量監控而非以T及B細胞為基準。The repopulated portion of this experiment was prematurely terminated when lymphocytes were 50-80% repopulated (depending on the dose), and lymphocyte repopulation was based on total lymphocyte count monitoring rather than T and B cells.

第65A-65E圖顯示在使用9D9-H10/K12(「9D9」)抗體投藥後72小時血液中CD4+T細胞、CD8+T細胞及B220+B細胞的含量。第66A-66E圖顯示在使用9D9-H10/K12(「9D9」)抗體投藥後72小時脾臟中CD4+T細胞、CD8+T細胞及B220+B細胞的含量。第67A-67F圖顯示在使用9D9-H10/K12(「9D9」)抗體投藥後2小時循環細胞介素位準。第68圖顯示在使用9D9-H10/K12(「9D9」)抗體投藥後循環淋巴細胞隨時間的再增殖。Figure 65A-65E shows the levels of CD4+ T cells, CD8+ T cells, and B220+ B cells in the blood 72 hours after administration with the 9D9-H10/K12 ("9D9") antibody. Panels 66A-66E show the levels of CD4+ T cells, CD8+ T cells, and B220+ B cells in the spleen 72 hours after administration with the 9D9-H10/K12 ("9D9") antibody. Figures 67A-67F show circulating interleukin levels 2 hours after administration of the 9D9-H10/K12 ("9D9") antibody. Figure 68 shows repopulation of circulating lymphocytes over time following administration of 9D9-H10/K12 ("9D9") antibody.

實例50:huCD52基因轉殖老鼠中抗-CD52抗體的消耗及再增殖之分析(2C3-SFD1/K12、12G6-SFD1/K11及9D9-H10/K12)Example 50: Analysis of consumption and repopulation of anti-CD52 antibodies in huCD52 transgenic mice (2C3-SFD1/K12, 12G6-SFD1/K11 and 9D9-H10/K12)

於huCD52基因轉殖老鼠中檢視Campath-1H及人類化2C3-SFD1/K12、12G6-SFD1/K11及9D9-H10/K12細胞株於不同劑量位準的消耗活性。將老鼠靜脈內注射0.1或1.0毫克/公斤抗體,給藥後兩小時,收集血清以潛在地檢查循環細胞介素位準。給藥後三天,殺死老鼠,及從每一隻老鼠收集血液及脾臟,以使用流式細胞計數法分析來測定細胞消耗位準。評估樣品以測定存在於huCD52基因轉殖老鼠的循環週邊血液或脾臟的總T輔助細胞(CD4+)、細胞毒性T細胞(CD8+)、B細胞(B220+)及骨髓樣的細胞子族群之相對數目。此外,執行T及B細胞子組分析以測定總消耗作用。當與經PBS治療之動物相較時,所有人類化抗體(2C3-SFD1/K12、12G6-SFD1/K11及9D9-H10/K12)媒介脾臟及血液內的淋巴細胞消耗。對所有抗體而言,於血液中較於脾臟中的消耗更為穩健,且於兩種組織中的消耗為劑量相依的。對CD4及CD8+T細胞而言消耗最顯著,且在B細胞部分係為較少的消耗。各種T及B細胞子組不同程度地消耗。自然T細胞(CD4與CD8兩者)與其他細胞族群(包含記憶性及T調節細胞)相較被證實為最大消耗,這些細胞族群係為較少程度地消耗。在B細胞部份,成熟B細胞較不成熟B細胞消耗更快速。血清細胞介素分析顯示在投藥後2小時IL-6、MCP-1及TNF 的位準顯著增加。對所有抗體(包含Campath-1H)皆觀察到上升,且為劑量相依增加(亦即對1.0毫克/公斤劑量位準所觀察到的細胞介素位準較0.1毫克/公斤劑量為高)。與Campath-1H相較,2C3-SFD1/K12及12G6-SFD1/K11誘發類似的IL-6位準,而9D9-H10/K12誘發IL-6至顯著較低位準。對MCP-1而言,12G6-SFD1/K11抗體誘發較低位準,及與Campath-1H相較而言,12G6-SFD1/K11與9D9-H10/K12兩者皆降低TNF位準。Examination of Campath-1H in huCD52 transgenic mice And humanized 2C3-SFD1/K12, 12G6-SFD1/K11 and 9D9-H10/K12 cell lines were consumed at different dose levels. Mice were injected intravenously with 0.1 or 1.0 mg/kg of antibody, and two hours after dosing, serum was collected to potentially examine circulating cytokine levels. Three days after the administration, the mice were sacrificed, and blood and spleen were collected from each mouse to determine the level of cell consumption using flow cytometry analysis. Samples were evaluated to determine the relative number of total T helper cells (CD4+), cytotoxic T cells (CD8+), B cells (B220+), and myeloid cell subpopulations present in the circulating peripheral blood or spleen of huCD52 gene-transferred mice. In addition, T and B cell subgroup analyses were performed to determine total depletion. All humanized antibodies (2C3-SFD1/K12, 12G6-SFD1/K11 and 9D9-H10/K12) were used to mediate lymphocytes in the spleen and blood when compared to PBS-treated animals. For all antibodies, consumption in the blood is more robust than in the spleen, and consumption in both tissues is dose dependent. The most significant consumption was for CD4 and CD8+ T cells, and less was consumed in the B cell fraction. Various T and B cell subgroups are consumed to varying degrees. Natural T cells (both CD4 and CD8) have been shown to be the most consumed compared to other cell populations (including memory and T regulatory cells), which are consumed to a lesser extent. In the B cell fraction, mature B cells consume more rapidly than immature B cells. Serum interleukin analysis showed a significant increase in the levels of IL-6, MCP-1 and TNF 2 hours after administration. For all antibodies (including Campath-1H Both were observed to increase and dose-dependently increased (ie, the level of interleukin observed at the 1.0 mg/kg dose level was higher than the 0.1 mg/kg dose). With Campath-1H In contrast, 2C3-SFD1/K12 and 12G6-SFD1/K11 induced a similar IL-6 level, while 9D9-H10/K12 induced IL-6 to a significantly lower level. For MCP-1, 12G6-SFD1/K11 antibody induced lower levels, and with Campath-1H In contrast, both 12G6-SFD1/K11 and 9D9-H10/K12 reduced TNF levels.

第69A-69D圖顯示在使用Campath-1H(「Campath」)、2C3-SFD1/K12(「2C3」)、12G6-SFD1/K11(「12G6」)、及9D9-H10/K12(「9D9」)抗體投藥後72小時,血液中總體淋巴細胞族群(CD4+T細胞、CD8+T細胞及B220+B細胞)及CD4+T細胞、CD8+T細胞及B220+B/NK細胞子型的含量。第70A-70D圖顯示在使用Campath-1H(「Campath」)、2C3-SFD1/K12(「2C3」)、12G6-SFD1/K11(「12G6」)、及9D9-H10/K12(「9D9」)抗體投藥後72小時,脾臟中總體淋巴細胞族群(CD4+ T細胞、CD8+ T細胞及B220+ B細胞)及CD4+ T細胞、CD8+ T細胞及B220+ B/NK細胞子型的含量。第71A-71F圖顯示在使用Campath-1H、2C3-SFD1/K12、12G6-SFD1/K11、及9D9-H10/K12抗體投藥後2小時循環細胞介素位準。Figure 69A-69D shows the use of Campath-1H ("Campath"), 2C3-SFD1/K12 ("2C3"), 12G6-SFD1/K11 ("12G6"), and 9D9-H10/K12 ("9D9") antibody 72 hours after administration of total lymphocytes in the blood The content of the population (CD4+ T cells, CD8+ T cells and B220+ B cells) and CD4+ T cells, CD8+ T cells and B220+B/NK cell subtypes. Figure 70A-70D shows the use of Campath-1H ("Campath"), 2C3-SFD1/K12 ("2C3"), 12G6-SFD1/K11 ("12G6"), and 9D9-H10/K12 ("9D9") antibody 72 hours after administration, total lymphocytes in the spleen The content of CD4+ T cells, CD8+ T cells and B220+ B cells, and CD4+ T cells, CD8+ T cells and B220+ B/NK cell subtypes. Figure 71A-71F shows the use of Campath-1H The 2C3-SFD1/K12, 12G6-SFD1/K11, and 9D9-H10/K12 antibodies were circulated for cytokine levels 2 hours after administration.

實例51:huCD52基因轉殖老鼠中抗-huCD52人類化9D9細胞株之直接比較(9D9H10/K12及9D9H11/K12)Example 51: Direct comparison of anti-huCD52 humanized 9D9 cell lines in huCD52 gene transgenic mice (9D9H10/K12 and 9D9H11/K12)

於huCD52基因轉殖老鼠中檢視兩種人類化抗-CD529D9細胞株(9D9-H10/K12及9D9-H11/K12)的消耗活性。將老鼠靜脈內注射0.1或1.0毫克/公斤抗體。給藥後三天,殺死老鼠,及從每一隻老鼠收集血液及脾臟,以使用流式細胞計數法分析來測定細胞消耗位準。評估樣品以測定存在於huCD52基因轉殖老鼠的循環週邊血液或脾臟的總T輔助細胞(CD4+)、細胞毒性T細胞(CD8+)、B細胞(B220+)及骨髓樣的NK細胞子族群之相對數目。以任一種抗體的治療於血液及脾臟中產生類似的淋巴細胞消耗,且淋巴細胞消耗於血液中較為穩健。而且,在兩者組織中CD4及CD8+ T細胞較B細胞及NK細胞更強烈消耗。儘管使用9D9-H10/K12細胞株的消耗較使用9D9-H11/K12細胞株的消耗似乎較不穩健,此差別並非統計上有意義的。The depletion activity of two humanized anti-CD529D9 cell lines (9D9-H10/K12 and 9D9-H11/K12) was examined in huCD52 gene-transfected mice. Rats were injected intravenously with 0.1 or 1.0 mg/kg of antibody. Three days after the administration, the mice were sacrificed, and blood and spleen were collected from each mouse to determine the level of cell consumption using flow cytometry analysis. Assess samples to determine the relative number of total T helper cells (CD4+), cytotoxic T cells (CD8+), B cells (B220+), and bone marrow-like NK cell subpopulations present in circulating peripheral blood or spleen of huCD52 gene-transferred mice. . Treatment with either antibody produces similar lymphocyte depletion in the blood and spleen, and lymphocytes are more stable in the blood. Moreover, CD4 and CD8+ T cells are more strongly consumed than B cells and NK cells in both tissues. Although the consumption of the 9D9-H10/K12 cell line appears to be less robust than the consumption of the 9D9-H11/K12 cell line, this difference is not statistically significant.

第72圖顯示在使用9D9-H10/K12及9D9-H11/K12抗體投藥後72小時血液中CD4+ T細胞、CD8+ T細胞、B220+ B細胞及NK細胞的含量。第73圖顯示在使用9D9-H10/K12及9D9-H11/K12抗體投藥後72小時脾臟中CD4+ T細胞、CD8+T細胞、B220+B細胞及NK細胞的含量。Figure 72 shows the levels of CD4+ T cells, CD8+ T cells, B220+ B cells, and NK cells in the blood 72 hours after administration with the 9D9-H10/K12 and 9D9-H11/K12 antibodies. Figure 73 shows the contents of CD4+ T cells, CD8+ T cells, B220+ B cells, and NK cells in the spleen 72 hours after administration with the 9D9-H10/K12 and 9D9-H11/K12 antibodies.

實例52:huCD52基因轉殖老鼠中抗-huCD52人類化12G6細胞株之直接比較(12G6-SFD1/K11及12G6-SFD1-K12)Example 52: Direct comparison of anti-huCD52 humanized 12G6 cell lines in huCD52 gene transgenic mice (12G6-SFD1/K11 and 12G6-SFD1-K12)

於huCD52基因轉殖老鼠中檢視兩種人類化抗-CD52 12G6細胞株(12G6-SFD1/K11及12G6-SFD1/K12)的消耗活性。將老鼠靜脈內注射0.1或1.0毫克/公斤抗體。給藥後兩小時,收集血清以潛在地檢查循環細胞介素位準。給藥後三天,殺死老鼠,及從每一隻老鼠收集血液及脾臟以使用流式細胞計數法分析測定細胞消耗位準。評估樣品以測定存在於huCD52基因轉殖老鼠的循環週邊血液或脾臟的總T輔助細胞(CD4+)、細胞毒性T細胞(CD8+)、B細胞(B220+)及骨髓樣的細胞子族群之相對數目。此外,執行T及B細胞子組分析以測定總消耗作用。投藥12G6-SFD1/K11抗體或12G6-SFD1/K12抗體導致血液內顯著位準的淋巴細胞消耗。該兩個細胞株的淋巴細胞消耗活性存在些微或是沒有任何差異。淋巴細胞消耗的形式為使得自然CD4及CD8+T細胞較記憶T細胞或T調節細胞更高程度地消耗。骨髓樣的不管細胞株(12G6-SFD1/K11或12G6-SFD1/K12)或是劑量,骨髓樣的細胞族群係為較少程度地消耗。此實驗未執行血清細胞介素分析。The depletion activity of two humanized anti-CD52 12G6 cell lines (12G6-SFD1/K11 and 12G6-SFD1/K12) was examined in huCD52 transgenic mice. Rats were injected intravenously with 0.1 or 1.0 mg/kg of antibody. Two hours after dosing, serum was collected to potentially examine circulating cytokine levels. Three days after the administration, the mice were sacrificed, and blood and spleen were collected from each mouse to determine the level of cell consumption using flow cytometry analysis. Samples were evaluated to determine the relative number of total T helper cells (CD4+), cytotoxic T cells (CD8+), B cells (B220+), and myeloid cell subpopulations present in the circulating peripheral blood or spleen of huCD52 gene-transferred mice. In addition, T and B cell subgroup analyses were performed to determine total depletion. Administration of 12G6-SFD1/K11 antibody or 12G6-SFD1/K12 antibody results in significant levels of lymphocyte depletion in the blood. There was little or no difference in lymphocyte depletion activity between the two cell lines. Lymphocyte depletion is in the form such that natural CD4 and CD8+ T cells are consumed to a greater extent than memory T cells or T regulatory cells. Bone marrow-like cell populations are consumed to a lesser extent regardless of the cell line (12G6-SFD1/K11 or 12G6-SFD1/K12) or dose. Serum interleukin analysis was not performed in this experiment.

第74A-74D圖顯示在使用12G6-SFD1/K11(「12G6 K11」)及12G6-SFD1/K12(「12G6 K12」)抗體投藥後72小時血液中CD4+T細胞、CD8+T細胞、B220+B/NK細胞、及骨髓樣的細胞的含量。第75A-75D圖顯示在使用12G6-SFD1/K11(「12G6 K11」)及12G6-SFD1/K12(「12G6 K12」)抗體投藥後72小時脾臟中CD4+ T細胞、CD8+ T細胞、B220+ B/NK細胞、及骨髓樣的細胞的含量。Figure 74A-74D shows CD4+ T cells, CD8+ T cells, B220+ in blood 72 hours after administration with 12G6-SFD1/K11 ("12G6 K11") and 12G6-SFD1/K12 ("12G6 K12") antibodies. The content of B/NK cells and bone marrow-like cells. Figure 75A-75D shows CD4+ T cells, CD8+ T cells, B220+ B/NK in the spleen 72 hours after administration with 12G6-SFD1/K11 ("12G6 K11") and 12G6-SFD1/K12 ("12G6 K12") antibodies. The content of cells and bone marrow-like cells.

實例53:huCD52基因轉殖老鼠中抗-huCD52人類化9D9細胞株之直接比較(9D9 H11/K12、9D9 H16/K13、及9D9 H18/K13)Example 53: Direct comparison of anti-huCD52 humanized 9D9 cell lines in huCD52 transgenic mice (9D9 H11/K12, 9D9 H16/K13, and 9D9 H18/K13)

三種人類化9D9抗體(9D9 H11/K12、9D9 H16/K13、及9D9 H18/K13)的消耗活性係於huCD52基因轉殖老鼠中比較。人類CD52基因轉殖老鼠以PBS處理而作為溶劑對照組,或是以1毫克/公斤或0.1毫克/公斤的每一個抗體注射。給藥後兩小時,收集血清以測定循環細胞介素位準。給藥後三天,殺死老鼠,並收集和處理週邊血液與脾臟,以進行流式細胞計數法分析。評估樣品以測定存在於huCD52基因轉殖老鼠的循環週邊血液或脾臟的總T輔助細胞(CD4+)、細胞毒性T細胞(CD8+)、B細胞(B220+)及骨髓樣的細胞子族群之相對數目。此外,執行T及B細胞子組分析以測定總消耗作用。所有9D9(9D9 H11/K12、9D9 H16/K13、及9D9 H18/K13)抗體媒介血液及脾臟中淋巴細胞及骨髓樣的細胞族群的細胞消耗至相似程度。觀察到血液中淋巴細胞及骨髓樣的細胞的消耗較在脾臟中更為穩健,9D9細胞株(9D9 H11/K12、9D9 H16/K13、及9D9 H18/K13)的消耗活性之比較證實9D9-H16/K13導致更穩健的消耗,接著為9D9-H18/K13及9D9-H11/K12。此對於脾臟中淋巴細胞於1毫克/公斤劑量最為明顯,其中9D9-H16/K13治療較其他細胞株(9D9-H18/K13及9D9-H11/K12)產生更高程度的消耗,而且,消耗之形式使得自然CD4及CD8+T細胞較記憶T細胞或T調節細胞更高程度地消耗,及使用9D9-H16/K13時B細胞族群有更高位準的消耗。骨髓樣的細胞族群較不受抗-CD52處理的影響,無論抗體(9D9-H11/K12、9D9-H16/K13、或9D9-H18/K13)細胞株或劑量。所分析的細胞介素中,於IL-6、TNF及MCP-1觀察到上升。注射後,對所有9D9細胞株(9D9-H11/K12、9D9-H16/K13、及9D9-H18/K13)在0.1及1.0毫克/公斤的劑量位準皆觀察到類似的IL6及MCP-1循環位準。使用循環TNF位準觀察到些微差別,其中9D9-H16/K13細胞株的注射於1.0毫克/公斤劑量產生中度增加。The depletion activity of the three humanized 9D9 antibodies (9D9 H11/K12, 9D9 H16/K13, and 9D9 H18/K13) was compared in huCD52 gene transgenic mice. Human CD52 gene-transferred mice were treated with PBS as a solvent control group or with 1 mg/kg or 0.1 mg/kg of each antibody. Two hours after dosing, serum was collected to determine circulating interleukin levels. Three days after the administration, the mice were sacrificed, and peripheral blood and spleen were collected and treated for flow cytometry analysis. Samples were evaluated to determine the relative number of total T helper cells (CD4+), cytotoxic T cells (CD8+), B cells (B220+), and myeloid cell subpopulations present in the circulating peripheral blood or spleen of huCD52 gene-transferred mice. In addition, T and B cell subgroup analyses were performed to determine total depletion. All 9D9 (9D9 H11/K12, 9D9 H16/K13, and 9D9 H18/K13) antibody mediator blood and spleen cells in lymphocytes and bone marrow-like cell populations were consumed to a similar extent. It was observed that the consumption of lymphocytes and bone marrow-like cells in the blood was more stable than in the spleen, and the comparison of the depletion activities of the 9D9 cell lines (9D9 H11/K12, 9D9 H16/K13, and 9D9 H18/K13) confirmed 9D9-H16. /K13 results in more robust consumption, followed by 9D9-H18/K13 and 9D9-H11/K12. This is the most obvious dose of 1 mg/kg for lymphocytes in the spleen, and 9D9-H16/K13 treatment produces a higher degree of consumption than other cell lines (9D9-H18/K13 and 9D9-H11/K12), and consumes The form allows natural CD4 and CD8+ T cells to be consumed to a greater extent than memory T cells or T regulatory cells, and a higher level of B cell population consumption when using 9D9-H16/K13. The bone marrow-like cell population is less affected by anti-CD52 treatment, regardless of antibody (9D9-H11/K12, 9D9-H16/K13, or 9D9-H18/K13) cell lines or doses. Among the interleukins analyzed, an increase was observed in IL-6, TNF, and MCP-1. Similar IL6 and MCP-1 cycles were observed at all doses of 0.1 and 1.0 mg/kg for all 9D9 cell lines (9D9-H11/K12, 9D9-H16/K13, and 9D9-H18/K13) after injection. Level. A slight difference was observed using circulating TNF levels, with a moderate increase in the injection of the 9D9-H16/K13 cell line at a dose of 1.0 mg/kg.

第76圖顯示在使用9D9-H11/K12、9D9-H16/K13、及9D9-H18/K13抗體投藥後72小時血液中總體淋巴細胞族群(CD4+T細胞、CD8+T細胞及B220+B細胞)的含量。第77A-77D圖顯示在使用9D9-H11/K12、9D9-H16/K13、及9D9-H18/K13抗體投藥後72小時血液中CD4+T細胞、CD8+T細胞、B220+B/NK細胞及骨髓樣的細胞子類型的含量。第78圖顯示在使用9D9 H11/K12、9D9 H16/K13、及9D9 H18/K13抗體投藥後72小時脾臟中總體淋巴細胞族群(CD4+T細胞、CD8+T細胞及B220+B細胞)的含量。第79A-79D圖顯示在使用9D9-H11/K12、9D9-H16/K13、及9D9-H18/K13抗體投藥後72小時脾臟中CD4+T細胞、CD8+ T細胞、B220+ B/NK細胞及骨髓樣的細胞子類型的含量。第80A-80F圖顯示在使用9D9-H11/K12、9D9-H16/K13、及9D9-H18/K13抗體投藥後2小時循環細胞介素位準。Figure 76 shows total lymphocyte populations in the blood (CD4+ T cells, CD8+ T cells, and B220+ B cells) 72 hours after administration with 9D9-H11/K12, 9D9-H16/K13, and 9D9-H18/K13 antibodies. The content of ). Figure 77A-77D shows CD4+ T cells, CD8+ T cells, B220+B/NK cells in the blood 72 hours after administration with 9D9-H11/K12, 9D9-H16/K13, and 9D9-H18/K13 antibodies. The content of bone marrow-like cell subtypes. Figure 78 shows the total lymphocyte population (CD4+ T cells, CD8+ T cells and B220+ B cells) in the spleen 72 hours after administration with 9D9 H11/K12, 9D9 H16/K13, and 9D9 H18/K13 antibodies. . Figure 79A-79D shows CD4+ T cells, CD8+ T cells, B220+ B/NK cells, and bone marrow samples in the spleen 72 hours after administration with 9D9-H11/K12, 9D9-H16/K13, and 9D9-H18/K13 antibodies. The content of the cell subtype. Panels 80A-80F show circulating interleukin levels 2 hours after administration with 9D9-H11/K12, 9D9-H16/K13, and 9D9-H18/K13 antibodies.

實例54:CD52基因轉殖老鼠中自2C3、12G6、及9D9家族之抗-CD52抗體的PK數據之分析Example 54: Analysis of PK data from anti-CD52 antibodies of the 2C3, 12G6, and 9D9 families in CD52 transgenic mice

人類化2C3-SFD1/K12、12G6-SFD1/K11、12G6-SFD1/K12、9D9-H16/K13及9D9-H18/K13的藥物動力數據係於huCD52基因轉殖老鼠中測定。將老鼠靜脈內注射1毫克/公斤的抗體,並在給藥後兩小時開始於各種時間點收集血液,每一個抗體的循環位準係使用抗-人類IgG ELISA評估。所計算半衰期為:2C3-SFD1/K12 79.0±23.9小時,12G6-SFD1/K11 49.0±14.4小時,12G6-SFD1/K12 75.1±28.5小時,9D9-H16/K13 59.8+26.6小時及9D9-H18/K13 42.2+15.7小時。The pharmacokinetic data for humanized 2C3-SFD1/K12, 12G6-SFD1/K11, 12G6-SFD1/K12, 9D9-H16/K13, and 9D9-H18/K13 were determined in huCD52 gene-transfected mice. Mice were intravenously injected with 1 mg/kg of antibody, and blood was collected at various time points starting two hours after administration, and the circulating level of each antibody was evaluated using an anti-human IgG ELISA. The calculated half-life is: 2C3-SFD1/K12 79.0±23.9 hours, 12G6-SFD1/K11 49.0±14.4 hours, 12G6-SFD1/K12 75.1±28.5 hours, 9D9-H16/K13 59.8+26.6 hours and 9D9-H18/K13 42.2 + 15.7 hours.

整體而言,在這些研究中揭露了顯著的動物間變異性。2C3-SFD1/K12及12G6-SFD1/K12的末相清除半衰期為類似的,儘管12G6-SFD1/K11的半衰期較短但沒有顯著差別。2C3-SFD1/K12的清除作用為最快速的,接著為12G6-SFD1/K11及12G6-SFD1/K12。對大部分所測量時間點而言,該兩個12G6處理為彼此相映的,而2C3-SFD1/K12顯示較少暴露及較快速清除。針對所有所測量PK參數,9D9-H16/K13及9D9-H18/K13為相當類似的。Overall, significant inter-animal variability was revealed in these studies. The terminal phase elimination half-lives of 2C3-SFD1/K12 and 12G6-SFD1/K12 were similar, although the half-life of 12G6-SFD1/K11 was short but not significantly different. The scavenging effect of 2C3-SFD1/K12 was the fastest, followed by 12G6-SFD1/K11 and 12G6-SFD1/K12. For most of the time points measured, the two 12G6 treatments were matched to each other, while 2C3-SFD1/K12 showed less exposure and faster clearance. 9D9-H16/K13 and 9D9-H18/K13 are quite similar for all measured PK parameters.

第81A-81B圖顯示給藥後血液中2C3-SFD1/K12、12G6-SFD1/K11、12G6-SFD1/K12、9D9-H16/K13及9D9-H18/K13抗體隨時間變化的位準。Figures 81A-81B show the levels of 2C3-SFD1/K12, 12G6-SFD1/K11, 12G6-SFD1/K12, 9D9-H16/K13, and 9D9-H18/K13 antibodies in the blood after administration.

實例55:因使用抗-CD52抗體治療造成之細胞介素暴發之評估Example 55: Evaluation of Interleukin Outbreaks Due to Treatment with Anti-CD52 Antibody

使用抗-CD52抗體治療之後血清細胞介素之釋出係於huCD52基因轉殖老鼠中評估。將動物以1毫克/公斤的Campath-1H、12G6-SFD1/K11、12G6-SFD1/K12、9D9-H16/K13或9D9-H18/K13治療。一組動物以5毫克/公斤的2C3-SFD1/K12治療,鑑於先前結果顯示以2C3-SFD1/K12注射相較於其他抗體會造成較低的消耗位準,於是基於達到類似消耗位準所需劑量來正常化該組動物。在治療後1、2、4、24及48小時,將所有群組放血及進行發炎細胞介素的CBA分析。在治療後3天殺死所有群組,並藉由流式細胞計數法針對脾臟中淋巴細胞的消耗而評估脾臟。以每一種抗體的治療產生各種標地物的消耗係類似於對Campath-1H所觀察到的。此對2C3-SFD1/K12亦為真,其中5毫克/公斤劑量係用於得到類似消耗。使用12G6-SFD1/K12及9D9-H16/K13觀察到於消耗的一些變化性,其大部分可能是因為動物的重複出血以得到為了細胞介素分析的血清。然而,對來自12G6(12G6-SFD1/K11及12G6-SFD1/K12)及9D9(9D9-H16/K13及9D9-H18/K13)家族成員的抗體而言,細胞介素表現減少,此在早期1及2小時時間點IL-6、MCP-1及TNF的釋出係為最顯著的。The release of serum interleukins after treatment with anti-CD52 antibody was assessed in huCD52 gene transgenic mice. Animals at 1 mg/kg of Campath-1H , 12G6-SFD1/K11, 12G6-SFD1/K12, 9D9-H16/K13 or 9D9-H18/K13 treatment. One group of animals was treated with 5 mg/kg of 2C3-SFD1/K12, and the previous results showed that the 2C3-SFD1/K12 injection resulted in a lower level of consumption compared to other antibodies, so it was based on achieving similar levels of consumption. The dose was used to normalize the animals in this group. All groups were bled and CBA analysis of inflammatory interleukins was performed at 1, 2, 4, 24, and 48 hours after treatment. All cohorts were sacrificed 3 days after treatment and spleens were assessed by flow cytometry for lymphocyte depletion in the spleen. The treatment of each of the antibodies produced a variety of landmarks similar to the Campath-1H Observed. This pair of 2C3-SFD1/K12 is also true, with a 5 mg/kg dose being used to achieve similar consumption. Some variability in consumption was observed with 12G6-SFD1/K12 and 9D9-H16/K13, most of which may be due to repeated bleeding of the animals to obtain serum for interleukin analysis. However, for antibodies from 12G6 (12G6-SFD1/K11 and 12G6-SFD1/K12) and 9D9 (9D9-H16/K13 and 9D9-H18/K13) family members, the expression of interleukins was reduced. The release profiles of IL-6, MCP-1 and TNF were most prominent at 2 hours.

第82A-82F圖顯示在使用Campath-1H(「Campath」)、12G6-SFD1/K11、12G6-SFD1/K12、9D9-H16/K13或9D9-H18/K13抗體給藥後於48-小時期間血液中細胞介素隨時間之含量。第83A-83E圖顯示在使用Campath-1H(「Campath」)、12G6-SFD1/K11、12G6-SFD1/K12、9D9-H16/K13或9D9-H18/K13抗體給藥後72小時於脾臟中總體淋巴細胞、CD4+ T細胞、CD8+ T細胞、B220+ B/NK細胞、及骨髓樣的細胞的含量。Figure 82A-82F shows the use of Campath-1H ("Campath"), 12G6-SFD1/K11, 12G6-SFD1/K12, 9D9-H16/K13 or 9D9-H18/K13 antibody content of interleukin in blood during 48-hour period. Figure 83A-83E shows the use of Campath-1H ("Campath"), 12G6-SFD1/K11, 12G6-SFD1/K12, 9D9-H16/K13 or 9D9-H18/K13 antibody, total lymphocytes, CD4+ T cells, CD8+ T cells in the spleen 72 hours after administration B220+ B/NK cells, and the content of bone marrow-like cells.

實例56:使用抗-CD52抗體的治療後的CD52基因轉殖老鼠血液中再增殖動力之評估Example 56: Evaluation of Reproliferative Motility in Blood of CD52 Gene Transgenic Mice after Treatment with Anti-CD52 Antibody

血液中許多細胞型式的再增殖動力於投藥人類化抗-CD52 2C3-SFD1/K12、9D9-H16/K13及12G6-SFD1/K12抗體之後予以評估。將老鼠靜脈內注射2毫克/公斤的每一抗體,以確保穩健的消耗位準,在注射後各種時間點,收集血液以進行流式細胞分析以測定血液中循環淋巴細胞位準,包含CD4+及CD8+ T細胞、調節T細胞、B細胞、NK細胞、嗜中性球及巨噬細胞。於注射後第3天,確認對每一個抗體在初始消耗活性未觀察到任何差別,於第一個月將老鼠每週抽血及之後每兩週抽血以監控再增殖動力。與Campath-1H相較,淋巴細胞再增殖動力與抗-CD52(2C3-SFD1/K12、9D9-H16/K13及12G6-SFD1/K12)抗體中的任一個類似。到第57天,B細胞回到血液中基礎線而T細胞到第84天接近基礎線位準。到第116天,CD8+T細胞尚未回到對照位準,但是隨著使用抗-CD52(2C3-SFD1/K12、9D9-H16/K13及12G6-SFD1/K12)抗體及Campath-1H的每一個,對所有被監控的其他細胞型式皆觀察到類似的再增殖動力。The repopulation motility of many cell types in the blood was assessed after administration of humanized anti-CD52 2C3-SFD1/K12, 9D9-H16/K13 and 12G6-SFD1/K12 antibodies. Rats were injected intravenously with 2 mg/kg of each antibody to ensure a robust level of consumption. At various time points after injection, blood was collected for flow cytometric analysis to determine circulating lymphocyte levels in the blood, including CD4+ and CD8+ T cells, regulatory T cells, B cells, NK cells, neutrophils and macrophages. On the third day after the injection, it was confirmed that no difference was observed in the initial consumption activity of each antibody, and the mice were bled weekly in the first month and blood was drawn every two weeks to monitor the repopulation power. With Campath-1H In contrast, lymphocyte repopulation kinetics are similar to any of the anti-CD52 (2C3-SFD1/K12, 9D9-H16/K13 and 12G6-SFD1/K12) antibodies. By day 57, B cells returned to the baseline in the blood and T cells approached the baseline level by day 84. By day 116, CD8+ T cells had not returned to the control level, but with anti-CD52 (2C3-SFD1/K12, 9D9-H16/K13 and 12G6-SFD1/K12) antibodies and Campath-1H Each of them was observed to have similar re-proliferation kinetics for all other cell types being monitored.

第84A-84G圖顯示在使用Campath-1H(「Campath」)、2C3-SFD1/K12、9D9-H16/K13及12G6-SFD1/K12抗體投藥之後,循環CD4+與CD8+T細胞、調節T細胞、B細胞、NK細胞、嗜中性球及巨噬細胞隨時間的再增殖。Figure 84A-84G shows the use of Campath-1H ("Campath"), 2C3-SFD1/K12, 9D9-H16/K13 and 12G6-SFD1/K12 antibodies, circulating CD4+ and CD8+ T cells, regulatory T cells, B cells, NK cells, neutrophils and Macrophages repopulate over time.

實例57:使用抗-CD52抗體之CD52基因轉殖老鼠中CD52表現之評估Example 57: Evaluation of CD52 expression in mice transfected with CD52 gene using anti-CD52 antibody

使用人類化抗-CD52抗體評估huCD52的表現以測定是否可於huCD52基因轉殖老鼠的成熟及發展中細胞族群觀察到類似的染色模式。2C3-SFD1/K12、12G6-SFD1/K11、12G6-SFD1/K12、9D9-H16/K13、及9D9-H18/K13抗體與FITC共軛以用於流式細胞染色。收集得自huCD52基因轉殖老鼠的組織並以染色處理。類似於Campath-1H,2C3-SFD1/K12、12G6-SFD1/K11、12G6-SFD1/K12、9D9-H16/K13、及9D9-H18/K13抗體染色來自基因轉殖老鼠之脾臟表現huCD52的淋巴細胞。該染色模式係為被發現於其他淋巴器官(例如胸腺及骨髓)的淋巴細胞族群及子組的代表。The performance of huCD52 was assessed using a humanized anti-CD52 antibody to determine if a similar staining pattern could be observed in the mature and developing cell population of huCD52 gene transgenic mice. 2C3-SFD1/K12, 12G6-SFD1/K11, 12G6-SFD1/K12, 9D9-H16/K13, and 9D9-H18/K13 antibodies were conjugated to FITC for flow cytometry. Tissues from huCD52 gene-transferred mice were collected and stained. Similar to Campath-1H , 2C3-SFD1/K12, 12G6-SFD1/K11, 12G6-SFD1/K12, 9D9-H16/K13, and 9D9-H18/K13 antibodies stained lymphocytes from spleen of gene-transgenic mice expressing huCD52. This staining pattern is representative of lymphocyte populations and subgroups found in other lymphoid organs such as the thymus and bone marrow.

第85圖顯示FITC-標記Campath-1H、2C3-SFD1/K12、12G6-SFD1/K11、12G6-SFD1/K12、9D9-H16/K13、及9D9-H18/K13抗體特定地結合至脾臟中huCD52淋巴細胞族群之能力。Figure 85 shows FITC-labeled Campath-1H The ability of 2C3-SFD1/K12, 12G6-SFD1/K11, 12G6-SFD1/K12, 9D9-H16/K13, and 9D9-H18/K13 antibodies to specifically bind to the huCD52 lymphocyte population in the spleen.

實例58:huCD52基因轉殖老鼠中使用抗-huCD52的單一劑量治療之直接比較Example 58: Direct comparison of single dose therapy with anti-huCD52 in huCD52 gene transgenic mice

數種人類化抗-CD52抗體(2C3-SFD1/K12、12G6-SFD1/K11、12G6-SFD1/K12、9D9-H16/K13及9D9-H18/K13)的消耗活性於huCD52基因轉殖老鼠中比較。將老鼠靜脈內注射1毫克/公斤抗體。給藥後兩小時,收集血清以進行細胞介素分析。三天後,殺死老鼠及收集血液和脾臟以比較淋巴細胞消耗位準。對所有抗-CD52抗體(2C3-SFD1/K12、12G6-SFD1/K11、12G6-SFD1/K12、9D9-H16/K13及9D9-H18/K13)都觀察到B及T細胞消耗的顯著位準,及與Campath-1H投藥之後所觀察到的那些係為可相比的。子組分析亦顯示在血液或脾臟中每一個抗體(2C3-SFD1/K12、12G6-SFD1/K11、12G6-SFD1/K12、9D9-H16/K13及9D9-H18/K13)的消耗位準沒有顯著差別。在注射Campath-1H之後,在IL-6及TNF兩者的循環位準有顯著增加。雖然每一個抗-CD52抗體(2C3-SFD1/K12、12G6-SFD1/K11、12G6-SFD1/K12、9D9-H16/K13及9D9-H18/K13)的注射產生較Campath-1H為顯著減少的TNF位準,IL-6的位準則為相似的。Comparison of the depletion activities of several humanized anti-CD52 antibodies (2C3-SFD1/K12, 12G6-SFD1/K11, 12G6-SFD1/K12, 9D9-H16/K13 and 9D9-H18/K13) in huCD52 transgenic mice . Rats were injected intravenously with 1 mg/kg of antibody. Two hours after administration, serum was collected for interleukin analysis. Three days later, the mice were killed and blood and spleen were collected to compare the levels of lymphocyte depletion. Significant levels of B and T cell consumption were observed for all anti-CD52 antibodies (2C3-SFD1/K12, 12G6-SFD1/K11, 12G6-SFD1/K12, 9D9-H16/K13, and 9D9-H18/K13). And with Campath-1H The ones observed after administration were comparable. Subgroup analysis also showed that the consumption level of each antibody (2C3-SFD1/K12, 12G6-SFD1/K11, 12G6-SFD1/K12, 9D9-H16/K13, and 9D9-H18/K13) was not significant in the blood or spleen. difference. Injecting Campath-1H Thereafter, there was a significant increase in the circulating level of both IL-6 and TNF. Although each anti-CD52 antibody (2C3-SFD1/K12, 12G6-SFD1/K11, 12G6-SFD1/K12, 9D9-H16/K13, and 9D9-H18/K13) was injected more than Campath-1H The positional criteria for IL-6 are similar for a significantly reduced TNF level.

第86A-86E圖顯示在使用Campath-1H(「Campath」)、2C3-SFD1/K12、12G6-SFD1/K11、12G6-SFD1/K12、9D9-H16/K13及9D9-H18/K13抗體投藥後72小時血液中總體淋巴細胞族群(CD4+T細胞、CD8+T細胞及B220+B細胞)及CD4+T細胞、CD8+T細胞、B220+B/NK細胞及骨髓樣的細胞子類型的含量。第87A87E圖顯示在使用Campath-1H(「Campath」)、2C3-SFD1/K12、12G6-SFD1/K11、12G6-SFD1/K12、9D9-H16/K13及9D9-H18/K13抗體投藥後72小時脾臟中總體淋巴細胞族群(CD4+T細胞、CD8+T細胞及B220+B細胞)及CD4+T細胞、CD8+T細胞、B220+B/NK細胞及骨髓樣的細胞子類型的含量。第88A-88C圖顯示在使用Campath-1H、2C3-SFD1/K12、12G6-SFD1/K11、12G6-SFD1/K12、9D9-H16/K13及9D9-H18/K13抗體投藥後2小時循環細胞介素位準。Figure 86A-86E shows the use of Campath-1H ("Campath"), 2C3-SFD1/K12, 12G6-SFD1/K11, 12G6-SFD1/K12, 9D9-H16/K13 and 9D9-H18/K13 antibodies in the blood 72 hours after administration of total lymphocyte population (CD4+T The content of cells, CD8+ T cells and B220+ B cells) and CD4+ T cells, CD8+ T cells, B220+ B/NK cells, and bone marrow-like cell subtypes. Figure 87A87E shows the use of Campath-1H ("Campath"), 2C3-SFD1/K12, 12G6-SFD1/K11, 12G6-SFD1/K12, 9D9-H16/K13 and 9D9-H18/K13 antibodies, total lymphocyte population in the spleen 72 hours after administration (CD4+T The content of cells, CD8+ T cells and B220+ B cells) and CD4+ T cells, CD8+ T cells, B220+ B/NK cells, and bone marrow-like cell subtypes. Figure 88A-88C shows the use of Campath-1H , 2C3-SFD1/K12, 12G6-SFD1/K11, 12G6-SFD1/K12, 9D9-H16/K13 and 9D9-H18/K13 antibodies were circulated for 2 hours after cytokine level.

實例59:使用抗-huCD52抗體單一劑量治療之後huCD52基因轉殖老鼠中淋巴細胞的深度消耗Example 59: Deep consumption of lymphocytes in huCD52 gene-transferred mice following single dose treatment with anti-huCD52 antibody

深度消耗分析係於使用抗-CD52 2C3-SFD1/K12、9D9-H16/K13及12G6-SFD1/K12抗體之huCD52基因轉殖老鼠中執行。將老鼠(N=4)靜脈內注射每一種抗體1毫克/公斤的單一劑量。三天後,殺死老鼠,並收集血液、脾臟、淋巴結及胸腺以使用多色流式細胞分析來比較淋巴細胞消耗位準。對所有抗-CD52 2C3-SFD1/K12、9D9-H16/K13及12G6-SFD1/K12抗體都觀察到顯著位準的B及T細胞消耗,且在所檢查的每一組織中,與那些在Campath-1H投藥之後所觀察到的係為可相比較的。子組分析亦顯示於在血液或脾臟中每一個抗體的消耗位準沒有顯著差別。於老鼠的淋巴結中亦觀察到顯著的淋巴細胞消耗位準,然而,在抗體活性方面顯示出有一些變異性,特別是當注意中樞性及效應記憶性T細胞子集時。因為關於LSR-II及CD8染色的技術議題,胸腺無法評估。Depletion analysis was performed in huCD52 gene transgenic mice using anti-CD52 2C3-SFD1/K12, 9D9-H16/K13 and 12G6-SFD1/K12 antibodies. Rats (N=4) were injected intravenously with a single dose of 1 mg/kg of each antibody. Three days later, mice were sacrificed and blood, spleen, lymph nodes, and thymus were collected to compare lymphocyte depletion levels using multicolor flow cytometry. Significant levels of B and T cell consumption were observed for all anti-CD52 2C3-SFD1/K12, 9D9-H16/K13, and 12G6-SFD1/K12 antibodies, and in each tissue examined, with those in Campath -1H The lines observed after administration were comparable. Subgroup analysis also showed no significant difference in the level of consumption of each antibody in the blood or spleen. Significant lymphocyte depletion levels were also observed in the lymph nodes of mice, however, there was some variability in antibody activity, especially when attention was paid to central and effector memory T cell subsets. Because of technical issues regarding LSR-II and CD8 staining, the thymus cannot be assessed.

第89A-89D圖顯示在使用Campath-1H(「Campath」)、2C3-SFD1/K12、9D9-H16/K13及12G6-SFD1/K12抗體投藥後72小時血液中CD4+T細胞、CD8+T細胞、B220+B細胞、及NK/骨髓樣的細胞子類型的含量。第90A-90D圖顯示在使用Campath-1H(「Campath」)、2C3-SFD1/K12、9D9-H16/K13及12G6-SFD1/K12抗體投藥後72小時脾臟中CD4+T細胞、CD8+T細胞、B220+B細胞及NK/骨髓樣的細胞子類型的含量。第91A-91D圖顯示在使用Campath-1H(「Campath」)、2C3-SFD1/K12、9D9-H16/K13及12G6-SFD1/K12抗體投藥後72小時淋巴結中CD4+T細胞、CD8+T細胞、B220+B細胞及NK/骨髓樣的細胞子類型的含量。Figure 89A-89D shows the use of Campath-1H ("Campath"), 2C3-SFD1/K12, 9D9-H16/K13 and 12G6-SFD1/K12 antibodies in blood 72 hours after administration of CD4+ T cells, CD8+ T cells, B220+ B cells, and NK/myeloid The content of the cell subtype. Figure 90A-90D shows the use of Campath-1H ("Campath"), 2C3-SFD1/K12, 9D9-H16/K13 and 12G6-SFD1/K12 antibodies were spleen CD4+ T cells, CD8+ T cells, B220+ B cells and NK/myeloid 72 hours after administration The amount of cell subtype. Figure 91A-91D shows the use of Campath-1H ("Campath"), 2C3-SFD1/K12, 9D9-H16/K13 and 12G6-SFD1/K12 antibodies were administered CD4+ T cells, CD8+ T cells, B220+ B cells and NK/myeloid in the lymph nodes 72 hours after administration. The amount of cell subtype.

實例60:huCD52基因敲入/基因剔除(KI/KO)基因轉殖老鼠於C57BL/6背景之產生及評估Example 60: Generation and evaluation of huCD52 knock-in/gene knockout (KI/KO) gene transfer mice in C57BL/6 background

一種新的人類CD52基因敲入/基因剔除老鼠模型於C57B1/6背景產生。為產生此老鼠,將老鼠CD52基因序列以人類CD52基因序列取代,使用標的策略以進行使用人類序列取代老鼠序列同時保持外顯子-內含子結構。使用一選擇標記以辨識包含新基因序列的後代。最終的對偶基因係由移除該選擇標記僅留下人類CD52基因序列而產生。A new human CD52 knock-in/gene knockout mouse model was generated in the C57B1/6 background. To generate this mouse, the mouse CD52 gene sequence was replaced with the human CD52 gene sequence, using the underlying strategy to replace the mouse sequence with the human sequence while maintaining the exon-intron structure. A selectable marker is used to identify progeny that contain the new gene sequence. The final dual gene line is produced by removing the selection marker leaving only the human CD52 gene sequence.

huCD52 KI/KO老鼠模型的基本特徵化涉及測定於淋巴細胞上人類CD52表現的程度,將自huCD52-KI/KO基因轉殖老鼠(N=4)及C57BL/6老鼠(N=2)的血液染色以進行hCD52表現,以及CD52分子/細胞的數目係使用Bang'S labs Simply Cellular抗-人類抗體試驗計算之。自 huCD52-KI/KO基因轉殖老鼠的週邊血液細胞之染色證實huCD52的表現於得自這些動物的淋巴細胞大多數係非常高的。表現位準類似於那些在人類CD4、CD8、及B細胞族群所觀察到的。於NK細胞及巨噬細胞的表現位準較對T細胞及B細胞所觀察到的為低。於這些老鼠的嗜中性球偵測到huCD52表現的增加位準,此與在人類嗜中性球或是來自於CD-1背景的原先基因轉殖老鼠系的類似細胞中減少的表現位準相反。類似的CD52表現位準於來自原先huCD52 CD1基因轉殖老鼠及huCD52 KI/KI老鼠的T及B細胞觀察到。The basic characterization of the huCD52 KI/KO mouse model involves measuring the extent of human CD52 expression on lymphocytes, transducing blood from huCD52-KI/KO gene (N=4) and C57BL/6 mice (N=2). Staining for hCD52 expression, and the number of CD52 molecules/cells were calculated using the Bang'S labs Simply Cellular anti-human antibody assay. Staining of peripheral blood cells from huCD52-KI/KO gene-transferred mice confirmed that huCD52 is expressed in very high numbers of lymphocytes derived from these animals. Performance levels are similar to those observed in human CD4, CD8, and B cell populations. The expression levels of NK cells and macrophages were lower than those observed for T cells and B cells. The neutrophil in these mice detected an increased level of huCD52 expression, which was reduced in performance levels in similar cells in human neutrophils or in the original gene-transgenic mouse line from the CD-1 background. in contrast. Similar CD52 expression levels were observed in T and B cells from the original huCD52 CD1 gene transgenic mice and huCD52 KI/KI mice.

第92A圖顯示huCD52-KI/KO及非-基因轉殖對照老鼠中於CD4+T細胞、CD8+T細胞、B220+B細胞、及NK/骨髓樣的細胞子形式的huCD52表現位準。第92B圖顯示huCD52-KI/KO及huCD52 CD1基因轉殖老鼠中於CD4+T細胞、CD8+T細胞、及B細胞的huCD52表現位準。Figure 92A shows the huCD52 expression levels in huCD52-KI/KO and non-gene transgenic control mice in CD4+ T cells, CD8+ T cells, B220+ B cells, and NK/myeloid cell subforms. Figure 92B shows the huCD52 expression levels of CD4+ T cells, CD8+ T cells, and B cells in huCD52-KI/KO and huCD52 CD1 gene transgenic mice.

實例61:12G6及2C3的小及大規模批次之間消耗特性的直接比較Example 61: Direct comparison of consumption characteristics between small and large batches of 12G6 and 2C3

將huCD52 KI/KO基因轉殖老鼠以12G6-SFD1/K12或2C3-SFD1/K12投藥以測定消耗活性。此外,使用Genzyme自兩個不同來源(小規模及大規模批次)產生的抗體檢查活性。將老鼠靜脈內注射每一種抗體1毫克/公斤,注射三天後,殺死老鼠,並收集血液以進行流式細胞分析以測定循環CD4+及CD8+T細胞、B細胞、NK細胞、嗜中性球及巨噬細胞的位準。於CD4T細胞、CD8+T細胞、B細胞、及NK細胞的消耗在小規模及大規模批次衍生抗體未觀察到有顯著差別。The huCD52 KI/KO gene was transfected into mice and administered with 12G6-SFD1/K12 or 2C3-SFD1/K12 to determine the depletion activity. In addition, the activity was examined using antibodies produced by Genzyme from two different sources (small scale and large batches). Rats were injected intravenously with 1 mg/kg of each antibody. Three days after the injection, the mice were sacrificed and blood was collected for flow cytometric analysis to determine circulating CD4+ and CD8+ T cells, B cells, NK cells, and neutrophils. The level of the ball and macrophages. The consumption of CD4 T cells, CD8+ T cells, B cells, and NK cells was not significantly different in small-scale and large-scale batch-derived antibodies.

亦藉由流式細胞計數法評估各種批次的12G6-SFD1/K12及2C3-SFD1/K12抗體,以比較於得自huCD52-KI/KO基因轉殖老鼠的脾細胞上的染色強度。12G6-SFD1/K12及2C3-SFD1/K12抗體於經分離的脾細胞上皆顯現與Campath-1H相同程度地辨識人類CD52。此外,在抗體的兩個來源(小規模及大規模批次)之間的辨識位準沒有任何差別。Various batches of 12G6-SFD1/K12 and 2C3-SFD1/K12 antibodies were also evaluated by flow cytometry to compare the staining intensity on spleen cells derived from huCD52-KI/KO gene-transferred mice. 12G6-SFD1/K12 and 2C3-SFD1/K12 antibodies are all expressed on the isolated splenocytes with Campath-1H Human CD52 was identified to the same extent. In addition, there is no difference in the level of identification between the two sources of antibodies (small scale and large batches).

第93A-93B圖顯示與Campath-1H對照組相較之結合至12G6-SFD1/K12與2C3-SFD1/K12抗體(來自各種製造來源)的huCD52。第94圖顯示在使用來自各種製造來源的12G6-SFD1/K12及2C3-SFD1/K12抗體投藥之後72小時血液中整體淋巴細胞族群(CD4+T細胞、CD8+T細胞、及B220+B細胞)的含量。Figure 93A-93B shows with Campath-1H The control group compared to huCD52 bound to 12G6-SFD1/K12 and 2C3-SFD1/K12 antibodies (from various manufacturing sources). Figure 94 shows the overall lymphocyte population (CD4+ T cells, CD8+ T cells, and B220+ B cells) in the blood 72 hours after administration of 12G6-SFD1/K12 and 2C3-SFD1/K12 antibodies from various manufacturing sources. The content.

實例62:huCD52-KI/KO基因轉殖老鼠中抗-CD52抗體之PK數據分析Example 62: PK data analysis of anti-CD52 antibodies in huCD52-KI/KO gene transgenic mice

人類化2C3-SFD1/K12、9D9-H16/K13及12G6-SFD1/K12抗體的藥物動力數據係於huCD52 KI/KO基因轉殖老鼠中測定。將老鼠靜脈內注射1毫克/公斤的抗體,及在給藥後兩小時開始於各種時間點收集血液,每一個抗體的循環位準係使用抗-人類IgG ELISA評估。對每一個人類化抗-CD52 2C3-SFD1/K12、9D9-H16/K13及12G6-SFD1/K12抗體而言,整體清除速率為類似,且2C3-SFD1/K12顯現潛在地較快速動力,而12G6-SFD1/K12存在於血清中最長的時間。The pharmacokinetic data for the humanized 2C3-SFD1/K12, 9D9-H16/K13 and 12G6-SFD1/K12 antibodies were determined in huCD52 KI/KO gene-transgenic mice. Mice were intravenously injected with 1 mg/kg of antibody, and blood was collected at various time points starting two hours after administration, and the circulating level of each antibody was evaluated using an anti-human IgG ELISA. For each of the humanized anti-CD52 2C3-SFD1/K12, 9D9-H16/K13, and 12G6-SFD1/K12 antibodies, the overall clearance rate was similar, and 2C3-SFD1/K12 showed potentially faster dynamics, while 12G6 -SFD1/K12 is present in serum for the longest period of time.

第95A-95B圖顯示在投藥後血液中2C3-SFD1/K12、9D9-H16/K13及12G6-SFD1/K12抗體隨時間之位準。Figure 95A-95B shows the level of 2C3-SFD1/K12, 9D9-H16/K13 and 12G6-SFD1/K12 antibodies in the blood over time after administration.

實例63:huCD52-KI/KO基因轉殖老鼠中12G6及2C3於EAE上預處理之評估Example 63: Evaluation of pretreatment of 12G6 and 2C3 on EAE in huCD52-KI/KO gene-transferred mice

抗-CD52抗體治療對於減少整體的疾病發生及實驗性自體免疫腦脊髓炎(EAE)的嚴重性之效果係於huCD52 KI/KO老鼠中評估。huCD52-KI/KO老鼠以2C3-SFD1/K12或12G6-SFD1/K12於第-5至-1天的期間處理。EAE(一種多發性硬化的模型)係經由使用於CFA中乳化的MOG35-55肽的免疫化而被誘發,及使用百日咳毒素於第0及2天處理。經媒劑處理的老鼠於注射後第10天開始顯示癱瘓徵狀,其發展為嚴重的惡化型疾病。相反地,使用2C3-SFD1/K12或12G6-SFD1/K12抗體預處理的老鼠延緩了疾病的開始並使整體疾病嚴重性降低。The effect of anti-CD52 antibody treatment on reducing overall disease development and the severity of experimental autoimmune encephalomyelitis (EAE) was assessed in huCD52 KI/KO mice. huCD52-KI/KO mice were treated with 2C3-SFD1/K12 or 12G6-SFD1/K12 during days -5 to -1 day. EAE, a model of multiple sclerosis, was induced by immunization of the MOG35-55 peptide emulsified in CFA, and treated with pertussis toxin on days 0 and 2. The vehicle-treated mice began to show signs of sputum on the 10th day after the injection, which progressed to a severely deteriorating disease. In contrast, mice pretreated with 2C3-SFD1/K12 or 12G6-SFD1/K12 antibodies delayed the onset of disease and reduced overall disease severity.

第96圖說明隨疾病惡化時間2C3-SFD1/K12及12G6-SFD1/K12的EAE臨床評分。Figure 96 illustrates the EAE clinical scores for 2C3-SFD1/K12 and 12G6-SFD1/K12 with disease progression time.

實例64:抗體的Fc修飾以變更抗-CD52抗體的藥物動力數據Example 64: Fc Modification of Antibodies to Change Drug Kinetic Data of Anti-CD52 Antibodies

抗體的Fc區域的改變係1)藉由變更與Fc受體的交互作用而影響抗體的生物活性,及/或2)藉由變更與FcRn新生受體的交互作用而影響抗體的藥物動力數據。FcRn分子係表現於血管內皮神經及被相信係為IgG循環的主要部位。FcRn結合至抗體Fc部份,其接著變成內化於細胞中。具有與FcRn高親和力交互作用的抗體會循環回到細胞表面及釋出回到循環,具低親和力交互作用的抗體在細胞內離解及最終降解。增加與FcRn交互作用的定點突變誘發產生與未經修飾抗體相較可維持在循環中較長時間的抗體。相反地,減少FcRn結合的抗體之Fc區域內的突變會縮短抗體的循環半衰期,已被敘述為會減少結合至FcRn造成較短循環半衰期的突變包含His435Ala單一突變及His310Ala/His435Gln雙突變(參考,例如,Kim等,"Mapping the site on human IgG for binding of the MHC class I-related receptor,FcRn," Eur. J. Immunol., 29:2819-2825(1999) and Kenanova等,「Tailoring the Pharmacokinetics and Positron Emission Tomography Imaging Properties of Anti-Carcinoembryonic Antigen Single-Chain Fv-Fc Antibody Fragments,」Cancer. Res. 65(2):622-631(2005))。The alteration of the Fc region of the antibody is 1) affecting the biological activity of the antibody by altering the interaction with the Fc receptor, and/or 2) affecting the pharmacokinetic data of the antibody by altering the interaction with the FcRn nascent receptor. The FcRn molecule is expressed in the vascular endothelial nerve and is believed to be the major site of the IgG cycle. FcRn binds to the Fc portion of the antibody, which in turn becomes internalized in the cell. Antibodies that interact with high affinity for FcRn circulate back to the cell surface and release back into the circulation, and antibodies with low affinity interactions dissociate and eventually degrade in the cell. Increased site-directed mutagenesis that interacts with FcRn induces antibodies that can be maintained in the circulation for longer periods of time than unmodified antibodies. Conversely, mutations in the Fc region of antibodies that reduce FcRn binding shorten the circulating half-life of antibodies, and mutations that have been described to reduce binding to FcRn resulting in shorter circulating half-lives include His435Ala single mutation and His310Ala/His435Gln double mutation (Reference, For example, Kim et al., "Mapping the site on human IgG for binding of the MHC class I-related receptor, FcRn," Eur. J. Immunol. , 29:2819-2825 (1999) and Kenanova et al., "Tailoring the Pharmacokinetics and Positron Emission Tomography Imaging Properties of Anti-Carcinoembryonic Antigen Single-Chain Fv-Fc Antibody Fragments," Cancer. Res. 65(2): 622-631 (2005)).

2C3-SFD1/K12抗體突變以產生具有經變更之PK數據的His435Ala2C3-SFD1/K12(「2C3-SFD1/K12-修飾1」)及His310Ala/His435Gln 2C3-SFD1/K12(「2C3-SFD1/K12-修飾2」)抗體。進行Biacore分析以確認至老鼠及人類FcRn分子的減少結合。Campath-1H及2C3-SFD1/K12抗體兩者以類似動力結合至每一個老鼠及人類FcRn分子。相反地,His435Ala 2C3-SFD1/K12抗體在低位準結合至老鼠FcRn但不結合至人類FcRn,His310Ala/His435Gln 2C3-SFD1/K12抗體並未結合至老鼠或人類FcRn分子,此顯示併入單或雙突變至2C3-SFD1/K12 Fc區域顯著地影響至老鼠及人類FcRn的結合。2C3-SFD1/K12 antibody mutation to generate His435Ala2C3-SFD1/K12 ("2C3-SFD1/K12-Modification 1") and His310Ala/His435Gln 2C3-SFD1/K12 with altered PK data ("2C3-SFD1/K12- Modification 2") antibody. Biacore analysis was performed to confirm reduced binding to mouse and human FcRn molecules. Campath-1H Both the 2C3-SFD1/K12 antibody binds to each mouse and human FcRn molecule with similar kinetics. In contrast, the His435Ala 2C3-SFD1/K12 antibody binds to mouse FcRn at a low level but does not bind to human FcRn, and the His310Ala/His435Gln 2C3-SFD1/K12 antibody does not bind to mouse or human FcRn molecules, which is shown to be incorporated into single or double Mutation to the 2C3-SFD1/K12 Fc region significantly affected binding to mouse and human FcRn.

第97A及97B圖說明Campath1H(「Campath」)、2C3-SFD1/K12(「2C3」)、His435Ala 2C3-SFD1/K12(「H435A 2C3」)及His310Ala/His435Gln 2C3-SFD1/K12(「H310A/H435Q 2C3」)結合至老鼠及人類FcRn分子之能力。Figures 97A and 97B illustrate Campath1H ("Campath"), 2C3-SFD1/K12 ("2C3"), His435Ala 2C3-SFD1/K12 ("H435A 2C3"), and His310Ala/His435Gln 2C3-SFD1/K12 ("H310A/H435Q 2C3") are integrated into mice and The ability of human FcRn molecules.

實例65:C57BI/6老鼠中靜脈內投藥之後經Fc修飾抗-CD52抗體的半衰期之評估Example 65: Evaluation of Half-Life of Fc-Modified Anti-CD52 Antibody After Intravenous Administration in C57BI/6 Mice

Fc修飾係併入2C3-SFD1/K12背脊骨以產生2C3-SFD1/K12-修飾1及2C3-SFD1/K12-修飾2抗體,所述抗體顯現出減少至負責維持抗體於循環中的FcRn受體的結合。測定2C3-SFD1/K12抗體及具減少的FcRn結合之2C3-SFD1/K12-修飾1及2C3-SFD1/K12-修飾2抗體的藥物動力數據。C57BL/6老鼠係用於在標的抗原(2C3-SFD1/K12結合至人類CD52但不與老鼠CD52交互反應)不存在下評估藥物動力數據。將老鼠靜脈內注射1毫克/公斤的抗體,於各種時間點收集血液以藉由ELISA分析老鼠血清中的循環人類IgG1位準。2C3-SFD1/K12-修飾1及2C3-SFD1/K12-修飾2抗體皆較2C3-SFD1/K12抗體快速地自血液中被清除。2C3-SFD1/K12具半衰期403小時,而2C3-SFD1/K12-修飾1具半衰期51小時及2C3-SFD1/K12-修飾2具半衰期8小時。2C3-SFD1/K12及2C3-SFD1/K12-修飾-1的 PK數據與1-室模型一致且僅為單相消除。相反地,2C3-SFD1/K12-修飾-2的數據與2室模型一致,具2個不同相的消除(在表中指定為α及β)。第一相持續直到投藥後48小時(α)及第二相(β,亦稱為末端消除項)於投藥後48小時開始。The Fc modification is incorporated into the 2C3-SFD1/K12 dorsal spine to produce 2C3-SFD1/K12-modified 1 and 2C3-SFD1/K12-modified 2 antibodies that appear to be reduced to the FcRn receptor responsible for maintaining the antibody in circulation. Combination of. Drug kinetic data for 2C3-SFD1/K12 antibodies and 2C3-SFD1/K12-modified 1 and 2C3-SFD1/K12-modified 2 antibodies with reduced FcRn binding were determined. C57BL/6 mice were used to assess drug motility data in the absence of the target antigen (2C3-SFD1/K12 binds to human CD52 but does not interact with mouse CD52). Mice were intravenously injected with 1 mg/kg of antibody, and blood was collected at various time points to analyze circulating human IgG1 levels in mouse serum by ELISA. Both the 2C3-SFD1/K12-modified 1 and 2C3-SFD1/K12-modified 2 antibodies were rapidly cleared from the blood compared to the 2C3-SFD1/K12 antibody. 2C3-SFD1/K12 has a half-life of 403 hours, while 2C3-SFD1/K12-modification 1 has a half-life of 51 hours and 2C3-SFD1/K12-modification 2 has a half-life of 8 hours. The PK data for 2C3-SFD1/K12 and 2C3-SFD1/K12-modification-1 are consistent with the 1-compartment model and are only single phase elimination. Conversely, the 2C3-SFD1/K12-modification-2 data is consistent with the 2-compartment model with 2 different phase eliminations (designated as alpha and beta in the table). The first phase continues until 48 hours after administration (α) and the second phase (β, also known as terminal elimination) begins 48 hours after administration.

第98圖顯示在非基因轉殖老鼠中2C3-SFD1/K12(「2C3未修飾」)、2C3-SFD1/K12-修飾1(「2C3-Fc突變體1」)及2C3-SFD1/K12-修飾2(「2C3-Fc突變體2」)的活體內清除作用。Figure 98 shows 2C3-SFD1/K12 ("2C3 unmodified"), 2C3-SFD1/K12-modified 1 ("2C3-Fc mutant 1") and 2C3-SFD1/K12-modification in non-gene-transferred mice 2 ("2C3-Fc mutant 2") in vivo clearance.

實例66:異型接合huCD52基因轉殖老鼠中於靜脈內投藥之後經Fc修飾之抗-CD52抗體的半衰期之評估Example 66: Evaluation of half-life of Fc-modified anti-CD52 antibody after intravenous administration in a heterozygous huCD52 gene transgenic mouse

測定2C3-SFD1/K12抗體與具活體外減少的FcRn結合之2C3-SFD1/K12-修飾1及2C3-SFD1/K12-修飾2抗體的藥物動力數據。huCD52基因轉殖老鼠係用於在2C3-SFD1/K12抗體標的抗原存在下評估PK數據。將老鼠靜脈內注射1毫克/公斤的抗體,於各種時間點收集血液以藉由ELISA測定老鼠血清中的循環人類IgG1位準。2C3-SFD1/K12-修飾1及2C3-SFD1/K12-修飾2抗體皆較2C3-SFD1/K12抗體快速地自血液中被清除。2C3-SFD1/K12具半衰期64小時,而2C3-SFD1/K12-修飾1具半衰期32小時,及2C3-SFD1/K12-修飾2具半衰期6.5小時。Drug kinetic data for 2C3-SFD1/K12-modified 1 and 2C3-SFD1/K12-modified 2 antibodies with 2C3-SFD1/K12 antibody binding to FcRn reduced in vitro were determined. The huCD52 gene transfer mouse line was used to evaluate PK data in the presence of the 2C3-SFD1/K12 antibody-labeled antigen. Mice were intravenously injected with 1 mg/kg of antibody, and blood was collected at various time points to measure circulating human IgG1 levels in mouse serum by ELISA. Both the 2C3-SFD1/K12-modified 1 and 2C3-SFD1/K12-modified 2 antibodies were rapidly cleared from the blood compared to the 2C3-SFD1/K12 antibody. 2C3-SFD1/K12 has a half-life of 64 hours, while 2C3-SFD1/K12-modification has a half-life of 32 hours, and 2C3-SFD1/K12-modification has a half-life of 6.5 hours.

第99圖顯示在huCD52基因轉殖老鼠中2C3-SFD1/K12(「2C3」)、2C3-SFD1/K12-修飾1(「2C3-Fc突變體1」)及2C3-SFD1/K12-修飾2(「2C3-Fc突變體2」)的活體內清除作用。Figure 99 shows 2C3-SFD1/K12 ("2C3"), 2C3-SFD1/K12-modification 1 ("2C3-Fc mutant 1") and 2C3-SFD1/K12-modification 2 in huCD52 gene-transferred mice ( In vivo clearance of "2C3-Fc mutant 2").

因為數據不足,未提供4.11、4.5、4.6、4.7、4.8、及4.9的PK參數。PK parameters of 4.11, 4.5, 4.6, 4.7, 4.8, and 4.9 were not provided because of insufficient data.

#-測試組為2C3-SFD1/K12(「2C3」)、2C3-SFD1/K12-修飾1(「2C3-M1」)及2C3-SFD1/K12-修飾2(「2C3-M2」)#-Test group is 2C3-SFD1/K12 ("2C3"), 2C3-SFD1/K12-Modification 1 ("2C3-M1") and 2C3-SFD1/K12-Modification 2 ("2C3-M2")

實例67:異型接合huCD52基因轉殖老鼠中靜脈內投藥經Fc修飾之抗-CD52抗體後活體內消耗之評估Example 67: Evaluation of in vivo consumption after intravenous administration of Fc-modified anti-CD52 antibody in a heterozygous huCD52 gene transgenic mouse

測定huCD52基因轉殖老鼠中2C3-SFD1/K12、2C3-SFD1/K12-修飾1、及2C3-SFD1/K12-修飾2抗體的消耗活性。將老鼠以1毫克/公斤的2C3-SFD1/K12、2C3-SFD1/K12-修飾1、或2C3-SFD1/K12-修飾2抗體處理及在72小時之後評估CD4 T細胞、CD8+T細胞、B細胞及NK細胞的存在。與投藥2C3-SFD1/K12抗體相較,投藥2C3-SFD1/K12-修飾1或2C3-SFD1/K12-修飾2抗體產生血液及脾臟中減少的消耗位準。而且,於血液及脾臟中2C3-SFD1/K12-修飾1皆顯示較2C3-SFD1/K12-修飾2為大的消耗。The depletion activity of 2C3-SFD1/K12, 2C3-SFD1/K12-modification 1, and 2C3-SFD1/K12-modified 2 antibodies in huCD52 gene-transfected mice was determined. The mice were treated with 1 mg/kg of 2C3-SFD1/K12, 2C3-SFD1/K12-modified 1, or 2C3-SFD1/K12-modified 2 antibody and evaluated for CD4 T cells, CD8+ T cells, B after 72 hours. The presence of cells and NK cells. Compared with the administration 2C3-SFD1 / K12 antibody administration 2C3 - SFD1 / K12- modification 1 or 2C3-SFD1 / K12- 2 modified antibodies in blood and spleen reduced consumption level. Moreover, 2C3-SFD1/K12-modification 1 in blood and spleen showed greater consumption than 2C3-SFD1/K12-modification 2.

第100A及100B圖顯示在使用2C3-SFD1/K12(「2C3」)、2C3-SFD1/K12-修飾1(「2C3-Fc突變體1」)及2C3-SFD1/K12-修飾2(「2C3-Fc突變體2」)抗體投藥之後72小時,血液及脾臟中整體淋巴細胞族群(CD4+T細胞、CD8+T細胞、B220+B細胞、及NK細胞)的含量。Figures 100A and 100B show the use of 2C3-SFD1/K12 ("2C3"), 2C3-SFD1/K12-modification 1 ("2C3-Fc mutant 1") and 2C3-SFD1/K12-modification 2 ("2C3- Fc mutant 2") The content of the whole lymphocyte population (CD4+ T cells, CD8+ T cells, B220+ B cells, and NK cells) in blood and spleen 72 hours after administration of the antibody.

實例68:人類化抗-CD52抗體的詳細抗原決定區專一性Example 68: Detailed epitope-specificity of humanized anti-CD52 antibodies

使用BiacoreT 100儀器決定人類化12G6-SFD1/K12、2C3-SFD1/K12、及9D9-H16/K13抗體的詳細抗原決定區專一性。做為對照,使用相同方法評估細胞株097(經純化之抗-人類CD52抗體,Biolegend)的抗原決定區專一性,先前已使用肽ELISA方法特徵化細胞株097的抗原決定區專一性(HaleG,"Synthetic peptide mimotype of the CAMPATH-1(CD52) antigen,a small glycosylphosphatidylinositol-anchored glycoprotein," Immunotechnology,1:175-187(1995))。在此Biacore T100試驗中,使用胺耦合直接固定抗體於Biacore CM5 Series S羧甲基葡聚糖感測晶片(GE#BR-1006-68)上,羧甲基葡聚糖表面係使用0.1莫耳濃度的N-羥基琥珀醯亞胺(NHS)及0.4莫耳濃度的N-乙基-N'-(3-二甲基胺基丙基)碳化二亞胺鹽酸鹽(EDC)的1:1混合物活化,使該表面可結合在抗體上的反應性胺基。因為與IgGs相較,IgM抗體傾向於具較高位準的非-特定結合,故同時研究老鼠IgMκ(mIgMκ)同種型對照(Biolegend clone #MM-30)的結合。抗體固定化之後,反應感測晶片表面係使用1莫耳濃度乙醇胺鹽酸鹽/NaOH pH 8.5淬熄,在每一個晶片上的一個流動室為空白參考表面,後續流動室以10,000 RU的抗體固定化。The specific epitope-specificity of the humanized 12G6-SFD1/K12, 2C3-SFD1/K12, and 9D9-H16/K13 antibodies was determined using the Biacore T 100 instrument. As a control, the epitope-specificity of cell line 097 (purified anti-human CD52 antibody, Biolegend) was evaluated by the same method, and the epitope-specificity of cell line 097 was previously characterized using a peptide ELISA method (HaleG, "Synthetic peptide mimotype of the CAMPATH-1 (CD52) antigen, a small glycosylphosphatidylinositol-anchored glycoprotein," Immunotechnology , 1:175-187 (1995)). In this Biacore T100 assay, an amine-coupled direct immobilization antibody was used on a Biacore CM5 Series S carboxymethyl dextran sensor wafer (GE#BR-1006-68) with a 0.1 molar carboxymethyldextran surface. Concentration of N-hydroxysuccinimide (NHS) and 0.4 molar concentration of N-ethyl-N'-(3-dimethylaminopropyl)carbodiimide hydrochloride (EDC) 1: 1 The mixture is activated such that the surface binds to reactive amine groups on the antibody. Since IgM antibodies tended to have higher levels of non-specific binding compared to IgGs, the binding of the mouse IgMκ (mIgMκ) isotype control (Biolegend clone #MM-30) was also investigated. After immobilization of the antibody, the surface of the reaction-sensing wafer was quenched using 1 molar concentration of ethanolamine hydrochloride/NaOH pH 8.5, one flow cell on each wafer was a blank reference surface, and the subsequent flow chamber was fixed with 10,000 RU of antibody. Chemical.

合成一系列包含人類CD52序列(MUT 1-MUT 12(分別為SEQ ID NOS: 169-180),表21)(參見,例如,Hale G,"Synthetic peptide mimotype of the CAMPATH-1(CD52)抗原、小糖基磷脂醯肌醇-錨定糖蛋白,"Immunotechnology,1:175-187(1995))的丙胺酸掃描突變肽。結合至這些突變CD52肽及結合至野生型CD52肽的抗體係於濃度500奈莫耳濃度、100奈莫耳濃度、50奈莫耳濃度、及0奈莫耳濃度測試。將肽稀釋至試驗流動緩衝液,HBS-EP+(10毫莫耳濃度HEPES、150毫莫耳濃度NaCl、0.05% P20表面活化劑、3毫莫耳濃度EDTA,pH 7.4)。亦包含100奈莫耳濃度樣品的複製。亦包含輕(κ)鏈特定鼠抗-老鼠IgM抗體(Southern Biotech Clone #1B4B1)做為IgM對照。T100儀器樣品室及試驗溫度係分別設定為4℃及25℃。人類CD52肽樣品以50微升/分鐘流速注入五分鐘以測量關聯性,及以50微升/分鐘流速於HBS-EP+中沖洗五分鐘以測量離解。抗體表面係使用10毫莫耳濃度甘胺酸-HCl pH 2.0於50微升/分鐘流速的六十秒注射剝除任何殘基的結合肽。分析係使用Biacore T100 Kinetics Evaluation軟體v2.0(GE Healthcare)執行,使用參考流動室及0奈莫耳濃度濃度差減(雙-參考差減)將數據相合至1:1模型。12G6-SFD1/K12抗體陰性((-),MUT 8)及陽性((+),MUT 9)肽抗原決定區辨識的代表性感應圖譜係分別示於第101A及第101B圖。所收編的肽結合數據係摘要於表21。A series of synthetic human CD52 sequences (MUT 1-MUT 12 (SEQ ID NOS: 169-180, respectively), Table 21) (see, for example, Hale G, "Synthetic peptide mimotype of the CAMPATH-1 (CD52) antigen, Small glycosylphospholipid phyto-inositol-anchored glycoprotein, " Immunological Technology , 1: 175-187 (1995)) Alanine scanning mutant peptide. The anti-systems bound to these mutant CD52 peptides and to the wild-type CD52 peptide were tested at a concentration of 500 nanomolar, 100 nanomolar, 50 nanomolar, and 0 nanomolar. The peptide was diluted to assay flow buffer, HBS-EP+ (10 millimolar concentration HEPES, 150 millimolar NaCl, 0.05% P20 surfactant, 3 millimolar EDTA, pH 7.4). A copy of the 100 nmerol concentration sample is also included. A light (k) chain specific mouse anti-mouse IgM antibody (Southern Biotech Clone #1B4B1) was also included as an IgM control. The T100 instrument sample chamber and test temperature were set to 4 ° C and 25 ° C, respectively. Human CD52 peptide samples were injected at a flow rate of 50 microliters per minute for five minutes to measure correlation and flushed in HBS-EP+ for five minutes at a flow rate of 50 microliters per minute to measure dissociation. The antibody surface was stripped of any residue binding peptide using a 10 millimolar concentration of glycine-HCl pH 2.0 at a flow rate of 50 microliters per minute for sixty seconds. The analysis was performed using Biacore T100 Kinetics Evaluation software v2.0 (GE Healthcare), and the data was combined to a 1:1 model using a reference flow chamber and 0 nmer concentration concentration subtraction (double-reference subtraction). Representative induction profiles for 12G6-SFD1/K12 antibody negative ((-), MUT 8) and positive ((+), MUT 9) peptide epitopes are shown in Figures 101A and 101B, respectively. The compiled peptide binding data lines are summarized in Table 21.

細胞株097的先前特徵化結合專一性(Hale G,"Synthetic peptide mimotype of the CAMPATH-1(CD52)antigen,a small glycosylphosphatidylinositol-anchored g1ycoprotein," Immunotechnology,1:175-187(1995))係由以包含人類CD52的C-端部分的六個殘基的肽塗佈ELISA培養盤以及接著測量抗體至該被固定肽的結合而測定。每一個殘基係由所有20個胺基酸所取代。因為在此ELISA中這些肽係接附於固體表面,所以該試驗較此處所敘述Biacore T100試驗(其使用固定於表面的抗體,且所述肽於該表面上流動)可能更受抗體親抗原性作用影響。在ELISA研究中,發現在成熟型式的人類CD52的位置11及12(分別為野生型殘基脯氨酸及絲胺酸)的丙胺酸取代會降低細胞株097至肽的強健結合,在此Biacore T100研究中,發現於位置11及12(及位置7、8、9、及10)的丙胺酸取代會廢去細胞株097的結合。ELISA試驗的假設性抗體親抗原性作用有可能是為何由ELISA方法所測定的細胞株097的對映抗原決定區較所敘述Biacore T100試驗所測定的為小之原因。The previously characterized specificity of cell line 097 (Hale G, "Synthetic peptide mimotype of the CAMPATH-1 (CD52) antigen, a small glycosylphosphatidylinositol-anchored g1ycoprotein," Immunotechnology , 1:175-187 (1995)) A peptide-coated ELISA plate containing six residues of the C-terminal portion of human CD52 and subsequent measurement of binding of the antibody to the immobilized peptide was determined. Each residue is replaced by all 20 amino acids. Since these peptides are attached to a solid surface in this ELISA, this assay may be more immunotropic than the Biacore T100 assay described herein, which uses antibodies immobilized on the surface and the peptides flow on the surface. Effect. In an ELISA study, alanine substitution at positions 11 and 12 of the mature human CD52 (wild-type residues valine and serine, respectively) was found to reduce the robust binding of cell line 097 to peptide, where Biacore In the T100 study, alanine substitution at positions 11 and 12 (and positions 7, 8, 9, and 10) was found to abolish the binding of cell line 097. The avidity of the hypothetical antibody in the ELISA assay may be the reason why the enantioselection region of cell line 097 as determined by the ELISA method is smaller than that determined by the described Biacore T100 assay.

2C3-SFD1/K12及12G6-SFD1/K12人類化抗體兩者至人類CD52肽序列的結合於位置7、8、及11對丙胺酸取代係為敏感的,以及人類化9D9-H16/K13的結合於位置4及11對丙胺酸取代係為敏感的。這些被定義的抗原決定區專一性與在實例4所觀察之結果重疊(摘要於表8)。不預期提供在結果之間的些微變化,因為在本個案中用於測量結合的Biacore T100方法與在實例4所使用方法顯著不同。與本個案相反,在實例4,所設計CHO細胞係用於表現人類CD52的野生型或丙胺酸-取代突變體。於此種哺乳動物細胞表現的人類CD52可為糖化的而影響結合,此並非用於在Biacore T100試驗中所使用的人類CD52之個案。The binding of both 2C3-SFD1/K12 and 12G6-SFD1/K12 humanized antibodies to the human CD52 peptide sequence is sensitive to alanine substitution at positions 7, 8, and 11, and the binding of humanized 9D9-H16/K13 Positions 4 and 11 are sensitive to alanine substitution. These defined epitope-specificities overlap with the results observed in Example 4 (summarized in Table 8). It is not expected to provide some slight variation between the results, as the Biacore T100 method used to measure binding in this case is significantly different from the method used in Example 4. In contrast to this case, in Example 4, the CHO cell line was designed to represent wild-type or alanine-substituted mutants of human CD52. Human CD52 expressed in such mammalian cells can be saccharified to affect binding, and this is not a case for human CD52 used in the Biacore T100 assay.

實例69:Campath-1H 或12G6-SFD1/K12所誘發的CD4+T細胞反應之評估 Example 69: Campath-1H Or evaluation of CD4+ T cell responses induced by 12G6-SFD1/K12

CD4+T細胞增生反應係在使用預先置入一組重疊15-mer肽(包含得自Campath-1H或人類化12G6-SFD1/K12抗體的變異區的序列)的自體移植樹突狀細胞(DC)的重複活體外刺激之後加以評估。這些實驗利用正常人類供給者T細胞及DCs,結果之測量係經由定量氘化胸腺嘧啶核苷合併響應經自體移植肽脈衝的抗原呈獻細胞(APC)而增生的人類CD4+T細胞。The CD4+ T cell proliferative response is pre-incorporated with a set of overlapping 15-mer peptides (included from Campath-1H) Or the sequence of autologous transplanted dendritic cells (DC) of humanized 12G6-SFD1/K12 antibody variant sequences was evaluated after repeated in vitro stimulation. These experiments utilized normal human donor T cells and DCs, and the results were measured by quantifying thymidine in combination with human CD4+ T cells that proliferated in response to autologous transplanted peptide-pulsed antigen-presenting cells (APCs).

細胞製備: 將PBMCs自得自BioMed SupplieS(Carlsbad,CA)的正常人類供給者分離術產品分離,供給者血液的HLA單倍型篩選係由Key BiologicS,LLC(Memphis,TN)執行(表22)。PBMCS係使用Ficoll-Paque PLUS密度梯度(GE Healthcare)及一系列使用磷酸生理食鹽水(PBS,Invitrogen,Carlsbad,CA)沖洗而分離,依循製造商建議流程使用Dynal CD4+珠基底陽性分離套組(Invitrogen)將CD4+T細胞自PBMC分離,將經分離CD4+T細胞冷凍於回收細胞培養冷凍介質(Invitrogen)並儲存於液態氮。樹突狀細胞(DC)係藉由使用GM-CSF(Leukine,Bayer,Leverkusin,Germany)及IL-4(Peprotech,Rocky Hill,NJ)析出附著性細胞六天而自PBMCS誘發,以GM-CSF及IL-4補充的介質於第4天置換,接著將DCs自燒瓶分離並冷凍於冷凍介質,接著轉移至液態氮儲存槽。 Cell preparation: PBMCs were isolated from normal human supplier isolation products from BioMed Supplie S (Carlsbad, CA) and HLA haplotype screening of donor blood was performed by Key BiologicS, LLC (Memphis, TN) (Table 22). PBMCS was isolated using a Ficoll-Paque PLUS density gradient (GE Healthcare) and a series of washes using phosphate physiological saline (PBS, Invitrogen, Carlsbad, CA), following the manufacturer's recommended procedure using the Dynal CD4+ bead-based positive separation kit (Invitrogen) CD4+ T cells were isolated from PBMC, and the isolated CD4+ T cells were frozen in a recovery cell culture freezing medium (Invitrogen) and stored in liquid nitrogen. Dendritic cells (DC) were induced from PBMCS by GM-CSF (Leukine, Bayer, Leverkusin, Germany) and IL-4 (Peprotech, Rocky Hill, NJ) to precipitate adherent cells for six days. The medium supplemented with IL-4 was replaced on day 4, and the DCs were separated from the flask and frozen in a freezing medium, followed by transfer to a liquid nitrogen storage tank.

包含Campath-1H及12G6-SFD1/K12的重及輕鏈變異區的肽係使用利用標準Fmoc-化學於CLEAR樹脂(Peptides International,Louisville,KY)的Rainin Symphony自動化肽合成器來合成。胺基酸(EMD Biosciences,San Diego,CA或Anaspec,San Jose,Ca)係以第三-丁氧羰基(BOC)、第三-丁基(tBu)、2,2,4,6,7-五甲基二氫-苯並呋喃-5-磺醯基(Pbf)、或三苯甲基(Trt)族群正交地保護。使用具莫耳比6:6:3:12:1的胺基酸/HCTU/HOBt/DIEA/樹脂執行耦合。在每一個循環期間,使用於DMF中的20%哌啶及2.5% 1,8-二氮雜雙環[5.4.0]十一-7-烯(DBU)溶液將Fmoc自胺基端移除,使用2.5%水的15毫升/0.1毫莫耳濃度樹脂/2.5% TIS/5%苯甲醚/90% TFA體積比的混合物執行自樹脂的去保護/裂解3小時,沉澱上層清液於二乙醚(-80℃)及於3000轉每分鐘製粒10分鐘,傾析乙醚及再次沖洗顆粒,接著冷凍乾燥粗肽。使用分析型HPLC(XBridge C18 4.5 x 100mm,Waters Corp.,Milford,MA)及MALDI-TOF質譜儀(Synapt,Waters Corp.,Milford,MA)驗證序列及評估純度,所有試劑為HPLC級(EMD Biosciences,San Diego,Ca or Sigma Aldrich,St. Louis,MO)。將經冷凍乾燥的肽再次懸浮於100% DMSO(Sigma)。將四十三個Campath-1H肽合併至11個直鏈組,每一組包含3或4個肽(表23:從上到下,輕鏈肽以SEQ ID NOs: 187-206表示,以及重鏈肽以SEQ ID NOs: 207-229表示)。42個12G6-SFD1/K12肽合併至8個直鏈組,每一組包含五或六個肽(表24:從上到下,輕鏈肽以SEQ ID NOs: 230-250表示,以及重鏈肽以SEQ ID NOs: 251-271表示)。 Peptide : Contains Campath-1H The peptides of the heavy and light chain variant regions of 12G6-SFD1/K12 were synthesized using a Rainin Symphony automated peptide synthesizer using standard Fmoc-chemistry in CLEAR resin (Peptides International, Louisville, KY). Amino acids (EMD Biosciences, San Diego, CA or Anaspec, San Jose, Ca) are based on a third-butoxycarbonyl (BOC), a third-butyl (tBu), 2, 2, 4, 6, 7- The pentamethyldihydro-benzofuran-5-sulfonyl (Pbf) or trityl (Trt) population is protected orthogonally. Coupling was performed using an amino acid/HCTU/HOBt/DIEA/resin with a molar ratio of 6:6:3:12:1. During each cycle, Fmoc was removed from the amine end using 20% piperidine in DMF and 2.5% 1,8-diazabicyclo [5.4.0] undec-7-ene (DBU) solution. Deprotection/cracking from the resin was carried out using a mixture of 2.5% water in a 15 ml/0.1 mmol concentration resin/2.5% TIS/5% anisole/90% TFA volume ratio for 3 hours, and the supernatant was precipitated in diethyl ether. (-80 ° C) and granulation at 3000 rpm for 10 minutes, decanting the ether and rinsing the particles again, followed by lyophilization of the crude peptide. Sequences and purity were verified using analytical HPLC (XBridge C18 4.5 x 100 mm, Waters Corp., Milford, MA) and MALDI-TOF mass spectrometer (Synapt, Waters Corp., Milford, MA), all reagents were HPLC grade (EMD Biosciences) , San Diego, Ca or Sigma Aldrich, St. Louis, MO). The lyophilized peptide was resuspended in 100% DMSO (Sigma). Will forty three Campath-1H The peptides were pooled into 11 linear groups, each containing 3 or 4 peptides (Table 23: top to bottom, light chain peptides are represented by SEQ ID NOs: 187-206, and heavy chain peptides are SEQ ID NOs: 207 -229 indicates). 42 12G6-SFD1/K12 peptides were combined into 8 linear groups, each containing five or six peptides (Table 24: top to bottom, light chain peptides represented by SEQ ID NOs: 230-250, and heavy chains) The peptide is represented by SEQ ID NOs: 251-271).

活體外刺激In vitro stimulation

DC抗原脈衝及成熟 在以肽處理前,將DCs融解,沖洗及析出於以5%人類血清(HS,Sigma,St. Louis,MO)、1%盤尼西尼-鏈黴素(Invitrogen,Carlsbad,CA)、100奈克/毫升GM-CSF、及20奈克/毫升IL-4補充的RPMI(Invitrogen,Carlsbad,CA),將DCs以2x105細胞/毫升在6-孔組織培養盤培養於4毫升介質,並使之於37℃附著1小時。在細胞附著之後,將10微克/毫升(總共40微克)的每一個肽加至包含DCs的孔,關聯於120微克或160微克的總肽加至每一個孔(Campath-1H 3-肽或4-肽群組),或200微克或240微克的總肽加至每一個孔(12G6-SFD1/K12 5-肽或6-肽群組)。將40微克的泛-DR結合抗原決定區(PADRE)加至DCs的一個孔並用做陽性對照,因為其可結合至大多數HLA-DR分子(Alexander J,等,"Development of high potency universal DR-restricted helper epitopes by modification of high affinity DR-blocking peptides,"Immunity,1:751-761(1994))。同樣地,將每一種都40微克的三種HLA-DR結合破傷風類毒素肽(DTIMMEPPYCKGLDIYYKA(SEQ ID NO: 183)、SAMLTNLIIFGPGPVLNKNEV(SEQ ID NO: 184)、及NNFTVSFWLRVPKVSASHLE(SEQ ID NO: 185))加至DCs的一個孔。類似地,熱滅活腺病毒係用做陽性抗原來源並將其以1微克/毫升加至DCs的一個孔。最後,DCs的一組維持不以抗原脈衝並用以做為「零」培育組。與各種抗原脈衝的DCs於37℃培養至少三小時,接著將DCs以包含50奈克/毫升TNF-α、10奈克/毫升IL-6,25奈克/毫升IL-1β(Peprotech,Rocky Hill,NJ)及500奈克/毫升PGE-2(Sigma Aldrich,St. Louis,MO)的'成熟細胞介素混合物'處理,接著使抗原脈衝DCs於37℃過夜成熟。 DC antigen pulse and maturation : DCs were thawed, washed and isolated before treatment with peptides in 5% human serum (HS, Sigma, St. Louis, MO), 1% penicillin-streptomycin (Invitrogen, Carlsbad, CA), 100 ng/ml GM-CSF, and 20 ng/ml IL-4 supplemented RPMI (Invitrogen, Carlsbad, CA), DCs were cultured in 6-well tissue culture plates at 2x10 5 cells/ml The medium was allowed to adhere to 4 ml and allowed to adhere at 37 ° C for 1 hour. After cell attachment, 10 μg/ml (40 μg total) of each peptide was added to wells containing DCs, and 120 μg or 160 μg total peptide was added to each well (Campath-1H) A total of 200 micrograms or 240 micrograms of total peptide was added to each well (the 12-G6-SFD1/K12 5-peptide or 6-peptide group). 40 micrograms of pan-DR binding epitope (PADRE) was added to one well of DCs and used as a positive control because it binds to most HLA-DR molecules (Alexander J, et al., "Development of high potency universal DR- Restricted helper epitopes by modification of high affinity DR-blocking peptides, " Immunity , 1:751-761 (1994)). Similarly, 40 micrograms of each of the three HLA-DR binding tetanus toxoid peptides (DTIMMEPPYCKGLDIYYKA (SEQ ID NO: 183), SAMLTNLIIFGPGPVLNKNEV (SEQ ID NO: 184), and NNFTVSFWLRVPKVSASHLE (SEQ ID NO: 185)) were added to A hole in the DCs. Similarly, heat inactivated adenovirus was used as a source of positive antigen and was added to one well of DCs at 1 μg/ml. Finally, a group of DCs was maintained not pulsed with antigen and used as a "zero" breeding group. DCs pulsed with various antigens were incubated at 37 ° C for at least three hours, followed by DCs containing 50 ng/ml TNF-α, 10 ng/ml IL-6, 25 ng/ml IL-1β (Peprotech, Rocky Hill) , NJ) and 500 ng/ml PGE-2 (Sigma Aldrich, St. Louis, MO) treatment of 'mature interleukin mixture', followed by antigen-pulsed DCs maturation at 37 °C overnight.

共-培養的建立 在肽裝載及成熟化之後,使用PBS洗DCs兩次,並使用以10% HS補充的4毫升RPMI再補足。融解自體移植CD4+T細胞並將其以2 x 106細胞/毫升再懸浮於以10% HS、盤尼西尼、及鏈黴素補充的RPMI,接著將DCs以10:1T細胞:DC比值(8 x 106 T細胞:8 x 105 DCs)於8毫升介質中使用自然CD4+T細胞培養。接著於37℃共-培養7天。在共-培養開始後約72小時,將細胞以25 IU重組IL-2(Peprotech,Rocky Hill,NJ)補充,及之後每3-4天進一步以25 IU重組IL-2於新介質中補充。 Establishment of co-culture : After peptide loading and maturation, DCs were washed twice with PBS and supplemented with 4 ml RPMI supplemented with 10% HS. Autologous transplantation of CD4+ T cells and resuspended at 2 x 10 6 cells/ml in RPMI supplemented with 10% HS, penicillin, and streptomycin, followed by DCs at 10:1 T cells: DC Ratio (8 x 10 6 T cells: 8 x 10 5 DCs) was cultured in 8 ml medium using natural CD4+ T cells. Then, it was co-cultured at 37 ° C for 7 days. About 72 hours after the start of the co-culture, the cells were supplemented with 25 IU of recombinant IL-2 (Peprotech, Rocky Hill, NJ), and then supplemented with 25 IU of recombinant IL-2 in new medium every 3-4 days.

共-培養的再刺激 在第7天(Stim #2)及第14天(Stim #3),共-培養依循下列步驟再刺激。 Co-culture re-stimulation : On day 7 (Stim #2) and day 14 (Stim #3), co-culture followed by the following steps to stimulate.

增生試驗:於5 x 105細胞/毫升於1毫升介質在24-孔低結合培養盤中,如上文所敘述析出、抗原脈衝及成熟DCs以易於細胞至U-底試驗培養盤的後續轉移。一種無關的HLA_DR結合肽,CS 378-398(肽序列DIEKKIAKMEKASSVFNVVNS(SEQ ID NO: 186)),係用做陰性對照(Alexander J,等,"Development of high potency universal DR-restricted helper epitopes by modification of high affinity DR-blocking peptides,"Immunity,1:751-761(1994))。在24小時DC熟化之後,使用冰冷PBS洗液將細胞自培養盤脫離,將DCs以1:1 T細胞:DC比值(2.5 x 104 DC/孔)與經抗原刺激T細胞培養於U-型底96孔培養盤,每一個T細胞群組使用以培育肽(特定反應)脈衝的DC及以不關連肽(非特定反應)脈衝的DC,以及僅T細胞及僅DC對照重覆試驗三次。在每孔加入1微Ci氘化胸腺嘧啶核苷(Perkin Elmer,Waltham,MA)之前進行試驗72小時,細胞於96孔培養盤收集器(Perkin Elmer)收集及所併入之氘化胸腺嘧啶核苷的量係經由於Wallac Microbeta Trilux計數器(Perkin Elmer)上測量CPM而定量。刺激指數係由將特定CPM除以非特定CPM而計算之。 Proliferation assay: 5 x 10 5 cells/ml in 1 ml medium in 24-well low-binding plates, as described above, antigenic pulses and mature DCs to facilitate subsequent transfer of cells to the U-bottom test plate. An unrelated HLA_DR binding peptide, CS 378-398 (peptide sequence DIEKKIAKMEKASSVFNVVNS (SEQ ID NO: 186)), used as a negative control (Alexander J, et al., "Development of high potency universal DR-restricted helper epitopes by modification of high Affinity DR-blocking peptides, " Immunity , 1:751-761 (1994)). After 24 hours of DC maturation, the cells were detached from the culture plate using ice-cold PBS wash, and DCs were cultured in U-type with antigen-stimulated T cells at a 1:1 T cell:DC ratio (2.5 x 10 4 DC/well). A bottom 96-well plate was used, each of which used a DC that incubated with a peptide (specific reaction) pulse and a DC that was pulsed with no related peptide (non-specific reaction), and a T cell and only a DC control repeated test three times. The assay was performed for 72 hours prior to the addition of 1 microCi deuterated thymidine (Perkin Elmer, Waltham, MA) per well, and the cells were collected in a 96-well culture plate collector (Perkin Elmer) and incorporated into the thymidine nucleus. The amount of glycoside was quantified by measuring CPM on a Wallac Microbeta Trilux counter (Perkin Elmer). The stimulus index is calculated by dividing a specific CPM by a non-specific CPM.

T細胞受體(TCR) V β用途: 將增生試驗建立後所留下的任何CD4+ T細胞冷凍以進行T細胞受體V β鏈表現的最後測定,融解細胞並依照製造商指示於IOTest Beta標示套組(Beckman Coulter,France)以辨識24種共軛Vβ族成員的抗體染色30分鐘,在以PBS沖洗及以1%甲醛補充之後,於FACScalibur(Becton Dickinson,Franklin Lakes,NJ)分析細胞,計算表現每一個被偵測的V-β鏈的細胞之百分率,如於第102圖及第103圖所摘要。 T cell receptor (TCR) V beta use: freeze any CD4+ T cells left after the establishment of the proliferation assay for final determination of T cell receptor V beta chain expression, melt the cells and label them according to the manufacturer's instructions on IOTest Beta. The kit (Beckman Coulter, France) stained for 24 minutes with antibodies recognizing 24 conjugated Vβ members, and after rinsing with PBS and supplemented with 1% formaldehyde, cells were analyzed in a FACScalibur (Becton Dickinson, Franklin Lakes, NJ). Percentage of cells expressing each of the detected V-beta chains, as summarized in Figures 102 and 103.

Campath-1H 致免疫性評估 Campath-1H Immunogenicity assessment

Campath-1H肽的致免疫性評估係如上文所敘述使用得自BioMedSupply(BMS)的十個正常供給者的PBMCs來執行,由刺激指數所顯示的反應摘要係描述於表25A。每一個供給者列於一行,及每一列列出用於刺激CD4+ T細胞的肽群組。刺激指數(SI)係經由將對培育肽群組的特定免疫反應除以非關連反應來測定,SI值<2.0則未列出。摘要於表25A的十個供給者中每一個的增生數據係報告於第104A-J圖。六個供給者顯現大於2.0的刺激指數,及結果稱之為'「Campath-1H反應者」。當使用兩個不同肽群組進行試驗時,自反應者其中一個的培育CD4+ T細胞,BMS352,顯現特定免疫反應。第七個供給者,BMS486,亦被分類為「反應者」,在此供給者,刺激指數為背景的1.7倍,其係以輕鏈肽群組986-989記錄。當評估此供給者內經培育T細胞培養的Vβ向上調節時,其顯示986-989經培育T細胞顯現單一Vβ(Vβ3)的高度向上調節(第102圖)。單一V β的向上調節及特定增生反應顯示BMS486為Campath-1H反應者,三個未-反應供給者,BMS200、BMS154、及BMS167,未顯示出增生數據或Vβ向上調節,此顯示肽特定免疫反應未發生。Campath-1H數據係定量為70%(7/10)反應者速率。引出免疫反應的肽群組總數為八,這八個免疫原性肽群組中的三個於具刺激指數3.0或更高的個別供給者引出強烈反應(表26)。Campath-1H The immunogenicity evaluation of the peptides was performed as described above using PBMCs from ten normal donors of BioMedSupply (BMS), and the reaction summaries shown by the stimulation index are described in Table 25A. Each supplier is listed in a row, and each column lists a peptide group used to stimulate CD4+ T cells. The stimulation index (SI) is determined by dividing the specific immune response to the cultured peptide group by a non-related reaction, with SI values < 2.0 not listed. The hyperplastic data for each of the ten suppliers in Table 25A is reported in Figures 104A-J. Six suppliers showed a stimulus index greater than 2.0, and the result was called 'Campath-1H Responder." When tested using two different peptide groups, one of the self-reactive ones incubated CD4+ T cells, BMS352, developed a specific immune response. The seventh supplier, BMS486, was also classified as a "reactor", where the stimulus index was 1.7 times the background, which was recorded as light chain peptide group 986-989. When the Vβ up-regulation of cultured T cell cultures in this supplier was evaluated, it showed that 986-989 showed a highly up-regulated single Vβ (Vβ3) by the cultured T cells (Fig. 102). Upward regulation of a single Vβ and specific proliferative responses indicate that BMS486 is Campath-1H Responders, three un-reactive donors, BMS200, BMS154, and BMS167, showed no proliferative data or up-regulation of V[beta], indicating that the peptide-specific immune response did not occur. Campath-1H The data was quantified to be 70% (7/10) responder rate. The total number of peptide groups that elicited an immune response was eight, and three of the eight immunogenic peptide groups elicited a strong response from individual donors with a stimulation index of 3.0 or higher (Table 26).

表25:刺激指數數據摘要Table 25: Summary of stimulus index data

實例70:由12G6-SFD1/K12所誘發CD4+T細胞反應之評估Example 70: Evaluation of CD4+ T cell responses induced by 12G6-SFD1/K12

12G6-SFD1/K12變異區的致免疫性評估及Vβ分析係如在實例69對Campath-1H所敘述的來執行,其使用得自十個正常供給者的細胞。摘要於表25B的該十個供給者中每一個的增生數據係報告於第105A-J圖。這十個供給者中的兩個亦用於上文所敘述之Campath-1H評估(BMS486及BMS484),而其餘八個僅以12G6-SFD1/K12肽測試。一個供給者,BMS484,對三個肽群組反應並被分類為「12G6-SFD1/K12反應者」(表25B)。兩個供給者,BMS927及BMS928,每一者皆對一個肽群組反應,而因此亦被分類為「反應者」。供給者BMS928對包含重鏈肽1066、1067、1068、1083、1084、及1085的群組顯示2.0的弱刺激指數,此反應可由分析增生T細胞對Vβ用途而確認。反應的BMS928T細胞顯現單一Vβ(Vβ20)的向上調節(第103圖)。供給者BMS927於使用一組輕鏈肽培育的T細胞中顯示2.5的刺激指數,反應的BMS927 T細胞的Vβ分析並未顯示相對於背景的單一Vβ向上調節。然而,此供給者保留在「反應者」類別,因為Vβ套組僅代表70%的所有可能Vβ用途。在這10個供給者的致免疫性的12G6-SFD1/K12速率為30%(3/10),少於Campath-1H反應者速率的一半(70%),總共五個肽群組引出反應,然而五個群組中沒有一個產生大於3.0的刺激指數(表26)。The immunogenicity assessment and Vβ analysis of the 12G6-SFD1/K12 variant was as in Example 69 for Campath-1H. Executed as described, which uses cells from ten normal suppliers. The proliferative data for each of the ten suppliers in Table 25B is reported in Figures 105A-J. Two of the ten suppliers are also used for the Campath-1H described above. The evaluations (BMS486 and BMS484) were evaluated while the remaining eight were tested only with the 12G6-SFD1/K12 peptide. One supplier, BMS484, reacted to three peptide groups and was classified as "12G6-SFD1/K12 Recipient" (Table 25B). Two suppliers, BMS927 and BMS928, each reacted to a peptide group and were therefore classified as "responders". The supplier BMS928 showed a weak stimulation index of 2.0 for the group comprising heavy chain peptides 1066, 1067, 1068, 1083, 1084, and 1085, which reaction was confirmed by analysis of proliferating T cells for Vβ use. The reacted BMS928T cells showed an upward regulation of a single Vβ (Vβ20) (Fig. 103). The supplier BMS927 showed a stimulation index of 2.5 in T cells incubated with a set of light chain peptides, and the Vβ analysis of the reacted BMS927 T cells did not show a single Vβ upregulation relative to the background. However, this supplier remains in the "Responders" category because the Vβ kit represents only 70% of all possible Vβ uses. The immunogenic 12G6-SFD1/K12 rate in these 10 suppliers was 30% (3/10), less than Campath-1H Half of the responder's rate (70%), a total of five peptide groups elicited a response, whereas none of the five cohorts produced a stimulation index greater than 3.0 (Table 26).

總結to sum up

與人類化抗-CD52單株抗體12G6-SFD1/K12的重及輕鏈變異區關聯的肽自十個供給者誘發較Campath-1H重及輕鏈變異區(70%)為少的免疫反應(30%),使用12G6-SFD1/K12所產生的CD4+ T細胞基礎免疫反應亦較Campath-1H所誘發的反應數值為小。Peptides associated with the heavy and light chain variant regions of humanized anti-CD52 monoclonal antibody 12G6-SFD1/K12 induced more than Campath-1H from ten donors The heavy and light chain variants (70%) were less immune (30%), and the CD4+ T cell basal immune response produced by 12G6-SFD1/K12 was also higher than that of Campath-1H. The value of the induced reaction is small.

下表列出本文中所使用的序列識別號碼。The table below lists the sequence identification numbers used in this article.

本文所引用的所有專利、公開申請案及參考文獻之意旨係以其全文併入做為參考。All patents, published applications and references cited herein are hereby incorporated by reference in their entirety.

儘管本發明已經由參考其實例具體實施例而特別地示出及敘述,熟知該技藝者將了解可進行各種型式和細節的變化而不偏離由所附申請專利範圍所包含的本發明範圍。Although the present invention has been particularly shown and described with reference to the specific embodiments thereof, it will be understood that

第1A-1B圖為一種新穎抗-CD52單株抗體的發展之示意表示。一般方案係說明於第1A圖及老鼠抗-人類CD52抗體株及其同種型的名稱係顯示於第1B圖。Figure 1A-1B is a schematic representation of the development of a novel anti-CD52 monoclonal antibody. The general protocol is shown in Figure 1A and the mouse anti-human CD52 antibody strain and its isotype are shown in Figure 1B.

第2圖為許多老鼠抗-人類CD52 κ輕鏈序列(SEQ ID NOS:1-13)的胺基酸序列之排列。Campath-1G為一種老鼠單株抗體,由此得到人類化Campath-1H抗體。Figure 2 is an alignment of the amino acid sequences of a number of mouse anti-human CD52 κ light chain sequences (SEQ ID NOS: 1-13). Campath-1G is a mouse monoclonal antibody, which results in a humanized Campath-1H antibody.

第3圖為許多老鼠抗-人類CD52重鏈序列(SEQ ID NOS:14-26)的胺基酸序列之排列。Campath-1G為一種老鼠單株抗體,由此得到人類化Campath-1H抗體。Figure 3 is an alignment of the amino acid sequences of a number of mouse anti-human CD52 heavy chain sequences (SEQ ID NOS: 14-26). Campath-1G is a mouse monoclonal antibody, which results in a humanized Campath-1H antibody.

第4圖為野生型CD52及10種突變體CD52蛋白(SEQ ID NOS: 104-114,自上到下)之排列。Figure 4 is an arrangement of wild type CD52 and 10 mutant CD52 proteins (SEQ ID NOS: 104-114, top to bottom).

第5A圖說明抗體4B10及7F11於表現CD52丙胺酸掃描突變體的細胞的基於-FACS的N-端結合數據。Figure 5A illustrates the FACS-based N-terminal binding data of antibodies 4B10 and 7F11 in cells expressing CD52 alanine scanning mutants.

第5B圖說明抗體CF1D12、3G7、9D9、5F7、4G7及11C11於表現CD52丙胺酸掃描突變體的細胞的基於-FACS的中間區域結合數據。Figure 5B illustrates the FFS-based intermediate region binding data for antibodies expressing CF52D12, 3G7, 9D9, 5F7, 4G7 and 11C11 in CD52 alanine scanning mutants.

第5C圖說明抗體Campath-1H("Campath 1H")、2C3、12G6、及23E6於表現CD52丙胺酸掃描突變體的細胞的基於-FACS的結合數據。Figure 5C illustrates the antibody Campath-1H ("Campath 1H"), 2C3, 12G6, and 23E6 are based on -FACS-based binding data for cells expressing CD52 alanine scanning mutants.

第5D圖說明使用嵌合單株抗體組探查的CD52 +/- N-鏈結醣化的免免疫墨點。Figure 5D illustrates the immunoglobulins of CD52 +/- N-linked glycosylation probed using a chimeric monoclonal antibody panel.

第6圖為一種顯示於在CHO-K1 CD52 #67細胞上篩選的各種嵌合抗-CD52抗體的1.5小時CDC試驗的結果之圖。結果顯示嵌合抗體4B10及7F11與Campath-1H("Campath 1H")相匹比或更佳。Figure 6 is a graph showing the results of a 1.5 hour CDC test of various chimeric anti-CD52 antibodies screened on CHO-K1 CD52 #67 cells. The results show that chimeric antibodies 4B10 and 7F11 and Campath-1H ("Campath 1H") is better than or better.

第7圖為一種顯示於在CHO-K1 CD52 #67細胞上篩選的各種CD52上嵌合IgG1抗體的14小時ADCC試驗的結果之圖。結果顯示嵌合抗體2C3及12G6與Campath-1H("Campath 1H")相匹比或更佳。Figure 7 is a graph showing the results of a 14-hour ADCC assay showing chimeric IgG1 antibodies on various CD52 screened on CHO-K1 CD52 #67 cells. The results showed that chimeric antibodies 2C3 and 12G6 and Campath-1H ("Campath 1H") is better than or better.

第8A-8C圖說明替代抗-CD52抗體及Campath-1H("C-1H")抗體至經定義人類淋巴細胞族群的比較結合。這些圖顯示由FACS試驗所篩選的嵌合抗體的結合能力之層系。至最右端的曲線證實最高結合能力,然而至最左端的曲線以較低親合力結合。Figure 8A-8C illustrates alternative anti-CD52 antibodies and Campath-1H ("C-1H") antibody to a comparative binding of defined human lymphocyte populations. These figures show the layer of binding ability of the chimeric antibodies screened by the FACS assay. The curve to the far right end confirms the highest binding capacity, whereas the curve to the leftmost end combines with a lower affinity.

第9A-9C圖為說明在以嵌合抗體7F11、8G3、23E6、12G6、4B10、或5F7、或是Campath-1H("Cam")投藥之後72小時血液中CD4 T細胞(第9A圖)、CD8 T細胞(第9B圖)及CD19 B細胞(第9C圖)的含量的圖。Figure 9A-9C shows the chimeric antibody 7F11, 8G3, 23E6, 12G6, 4B10, or 5F7, or Campath-1H. ("Cam") A graph of the content of CD4 T cells (Fig. 9A), CD8 T cells (Fig. 9B) and CD19 B cells (Fig. 9C) in the blood 72 hours after administration.

第10A-10C圖為說明在以嵌合抗體7F11、8G3、23E6、12G6、4B10、或5F7、或是Campath-1H("Cam")投藥之後72小時脾臟中CD4 T細胞(第10A圖)、CD8 T細胞(第10B圖)及CD19 B細胞(第10C圖)的含量的圖。Figure 10A-10C shows the chimeric antibody 7F11, 8G3, 23E6, 12G6, 4B10, or 5F7, or Campath-1H. ("Cam") A graph of the content of CD4 T cells (Fig. 10A), CD8 T cells (Fig. 10B) and CD19 B cells (Fig. 10C) in the spleen 72 hours after administration.

第11A-11C圖為顯示在以嵌合抗體2C3、9D9、4B10、3G7、或11C11、或是Campath-1H("Cam")投藥之後72小時血液中CD4 T細胞(第11A圖)、CD8 T細胞(第11B圖)及CD19B細胞(第11C圖)的含量的圖。Figure 11A-11C shows the chimeric antibody 2C3, 9D9, 4B10, 3G7, or 11C11, or Campath-1H ("Cam") A graph of the content of CD4 T cells (Fig. 11A), CD8 T cells (Fig. 11B) and CD19B cells (Fig. 11C) in the blood 72 hours after administration.

第12圖為一種說明在使用7F11、4B10、或12G6嵌合單株抗體、或是Campath-1H("Campath")處理後存活老鼠百分率的Kaplan Meier存活圖。Figure 12 is a diagram showing the use of 7F11, 4B10, or 12G6 chimeric monoclonal antibodies, or Campath-1H. ("Campath") Kaplan Meier survival plot of percent of surviving mice after treatment.

第13圖為一種說明在使用2C3、8G3、或23E6嵌合單株抗體、或是Campath-1H("Campath")處理後存活老鼠百分率的Kaplan Meier存活圖。Figure 13 is a diagram showing the use of 2C3, 8G3, or 23E6 chimeric monoclonal antibodies, or Campath-1H. ("Campath") Kaplan Meier survival plot of percent of surviving mice after treatment.

第14圖為一種說明在使用9D9或4B10嵌合單株抗體、或是Campath-1H("Campath")處理後存活老鼠百分率的Kaplan Meier存活圖。Figure 14 is an illustration of the use of 9D9 or 4B10 chimeric monoclonal antibodies, or Campath-1H ("Campath") Kaplan Meier survival plot of percent of surviving mice after treatment.

第15圖為一種說明在使用2C3或11C11嵌合單株抗體、或是Campath-1H("Campath")處理後存活老鼠百分率的Kaplan Meier存活圖。Figure 15 is a diagram showing the use of 2C3 or 11C11 chimeric monoclonal antibodies, or Campath-1H. ("Campath") Kaplan Meier survival plot of percent of surviving mice after treatment.

第16圖為一種具最符合人類生殖株序列(SEQ ID NO: 97)的老鼠抗-人類CD52抗體4B10重鏈變異區(SEQ ID NO: 96)序列及人類化重鏈變異區序列(SEQ ID NO: 98)之排列。亦示出的是具最符合人類生殖株序列(SEQ ID NO: 100)的老鼠抗-人類CD52抗體4B10輕鏈變異區(SEQ ID NO: 99)序列及人類化輕鏈變異區序列(SEQ ID NO: 101)之排列。Figure 16 is a sequence of the mouse anti-human CD52 antibody 4B10 heavy chain variant region (SEQ ID NO: 96) and the humanized heavy chain variant region sequence (SEQ ID NO: 97). NO: 98). Also shown is the mouse anti-human CD52 antibody 4B10 light chain variant region (SEQ ID NO: 99) sequence and humanized light chain variant region sequence (SEQ ID NO: 100) that best fits the human reproductive strain sequence (SEQ ID NO: 100). NO: 101).

第17圖顯示人類化4B10重鏈(SEQ ID NO:103)及輕鏈(SEQ ID NO:102)變異區序列。Figure 17 shows the sequence of the humanized 4B10 heavy chain (SEQ ID NO: 103) and light chain (SEQ ID NO: 102) variant regions.

第18圖為一種顯示人類化抗體4B10-H1/K1("4B10-人類化")及嵌合抗體4B10相當地結合至表現CD52的細胞的圖。Figure 18 is a diagram showing that humanized antibody 4B10-H1/K1 ("4B10-humanized") and chimeric antibody 4B10 bind fairly to cells expressing CD52.

第19圖為一種顯示人類化抗體4B10-H1/K1("4B10-人類化")及嵌合抗體4B10媒介相當ADCC活性於表現CD52的細胞的圖。Figure 19 is a diagram showing that humanized antibody 4B10-H1/K1 ("4B10-humanized") and chimeric antibody 4B10 media equivalent ADCC activity to cells expressing CD52.

第20圖為一種顯示人類化抗體4B10-H1/K1("4B10-人類化")及嵌合抗體4B10媒介相當CDC活性於表現CD52的細胞的圖。Figure 20 is a diagram showing that humanized antibody 4B10-H1/K1 ("4B10-humanized") and chimeric antibody 4B10 media equivalent CDC activity to cells expressing CD52.

第21圖為一種說明嵌合抗-CD52抗體(12G6、7F11及4B10)、Campath-1H("Campath")、及人類化抗-CD52抗體4B10-H1/K1("4B10人類化(H1/K1)")於異型接合的huCD52基因轉殖老鼠的藥物動力數據的圖。Figure 21 is a diagram showing the chimeric anti-CD52 antibodies (12G6, 7F11 and 4B10), Campath-1H ("Campath"), and a map of pharmacokinetic data of humanized anti-CD52 antibody 4B10-H1/K1 ("4B10 humanized (H1/K1)") in a heterozygous huCD52 gene-transferred mouse.

第22A-22C圖為一種顯示在使用嵌合抗體4B10或人類化抗體4B10-H1/K1("4B10-Hu")或Campath-1H("Cam path")投藥之後72小時血液中CD4 T細胞(第22A圖)、CD8 T細胞(第22B圖)及CD19 B細胞(第22C圖)的含量的圖。Figure 22A-22C is a diagram showing the use of chimeric antibody 4B10 or humanized antibody 4B10-H1/K1 ("4B10-Hu") or Campath-1H ("Cam path") A graph of the content of CD4 T cells (Fig. 22A), CD8 T cells (Fig. 22B) and CD19 B cells (Fig. 22C) in the blood 72 hours after administration.

第23圖為一種顯示抗-CD52單株抗體的相對結合親合力之摘要的圖。Figure 23 is a graph showing a summary of the relative binding affinities of anti-CD52 monoclonal antibodies.

第24圖顯示人類化7F11重及輕(κ)鏈變異區序列。回復突變為老鼠殘基的胺基酸殘基加底線及CDR以粗體表示。Figure 24 shows the sequence of the humanized 7F11 heavy and light (κ) chain variant region. The amino acid residues that are back-mutated to the mouse residues are underlined and the CDRs are shown in bold.

第25圖為一種顯示嵌合及人類化7F11抗體相當地結合至表現CD52的細胞的統計表。X軸表示由所結合抗-CD52抗體所放出的螢光,其中每一個峰的面積表示總細胞族群。Figure 25 is a statistical table showing that chimeric and humanized 7F11 antibodies bind fairly to cells expressing CD52. The X-axis represents the fluorescence emitted by the bound anti-CD52 antibody, wherein the area of each peak represents the total cell population.

第26A圖顯示人類化2C3重鏈變異區序列。回復突變為老鼠殘基的胺基酸殘基加底線及CDR以粗體表示的圖。第26B圖顯示人類化2C3輕(κ)鏈變異區序列。回復突變為老鼠殘基的胺基酸殘基加底線及CDR以粗體表示。Figure 26A shows the sequence of the humanized 2C3 heavy chain variant region. The back mutation is a map showing the amino acid residue of the mouse residue plus the bottom line and the CDR in bold. Figure 26B shows the sequence of the humanized 2C3 light (κ) chain variant region. The amino acid residues that are back-mutated to the mouse residues are underlined and the CDRs are shown in bold.

第27A圖為一種顯示人類化及嵌合2C3抗體結合至表現CD52的細胞的統計表。X軸表示由所結合抗-CD52抗體所放出的螢光,其中每一個峰的面積表示總細胞族群。第27B圖為一種顯示嵌合及人類化2C3抗體的子群相當地結合至表現CD52的細胞的統計表。X軸表示由所結合抗-CD52抗體所放出的螢光,其中每一個峰的面積表示總細胞族群。Figure 27A is a statistical table showing the binding of humanized and chimeric 2C3 antibodies to cells expressing CD52. The X-axis represents the fluorescence emitted by the bound anti-CD52 antibody, wherein the area of each peak represents the total cell population. Figure 27B is a statistical table showing that a subpopulation of chimeric and humanized 2C3 antibodies binds fairly to cells expressing CD52. The X-axis represents the fluorescence emitted by the bound anti-CD52 antibody, wherein the area of each peak represents the total cell population.

第28A圖顯示人類化12G6重鏈變異區序列。回復突變為老鼠殘基的胺基酸殘基加底線及CDR以粗體表示。第28B圖顯示人類化12G6輕(κ)鏈變異區序列。回復突變為老鼠殘基的胺基酸殘基加底線及CDR以粗體表示。Figure 28A shows the sequence of the humanized 12G6 heavy chain variant region. The amino acid residues that are back-mutated to the mouse residues are underlined and the CDRs are shown in bold. Figure 28B shows the sequence of the humanized 12G6 light (κ) chain variant region. The amino acid residues that are back-mutated to the mouse residues are underlined and the CDRs are shown in bold.

第29圖為一種顯示嵌合及人類化12G6抗體的子群相當地結合至表現CD52的細胞的統計表。X軸表示由所結合抗-CD52抗體所放出的螢光,其中每一個峰的面積表示總細胞族群。Figure 29 is a statistical table showing that a subgroup of chimeric and humanized 12G6 antibodies binds fairly to cells expressing CD52. The X-axis represents the fluorescence emitted by the bound anti-CD52 antibody, wherein the area of each peak represents the total cell population.

第30A圖顯示人類化9D9重鏈變異區序列。回復突變為老鼠殘基的胺基酸殘基加底線及CDR以粗體表示的圖。第30B圖顯示人類化9D9輕(κ)鏈變異區序列。回復突變為老鼠殘基的胺基酸殘基加底線及CDR以粗體表示。Figure 30A shows the sequence of the humanized 9D9 heavy chain variant region. The back mutation is a map showing the amino acid residue of the mouse residue plus the bottom line and the CDR in bold. Figure 30B shows the sequence of the humanized 9D9 light (kappa) chain variant region. The amino acid residues that are back-mutated to the mouse residues are underlined and the CDRs are shown in bold.

第31圖為一種顯示嵌合及人類化9D9抗體的子群相當地結合至表現CD52的細胞的統計表。X軸表示由所結合抗-CD52抗體所放出的螢光,其中每一個峰的面積表示總細胞族群。Figure 31 is a statistical table showing that a subgroup of chimeric and humanized 9D9 antibodies binds fairly to cells expressing CD52. The X-axis represents the fluorescence emitted by the bound anti-CD52 antibody, wherein the area of each peak represents the total cell population.

第32A圖顯示Campath-1H("C1H")、嵌合2C3抗體、及人類化2C3-SFD1/K12抗體至初代人類T細胞及huCD52基因轉殖老鼠T細胞的結合曲線。第32B圖顯示Campath-1H("C1H")、嵌合9D9抗體、及人類化9D9抗體至初代人類T細胞及huCD52基因轉殖老鼠T細胞的結合曲線。第32C圖顯示Campath-1H("C1H")、嵌合12G6抗體及人類化12G6抗體至初代人類T細胞及huCD52基因轉殖老鼠T細胞的結合曲線。Figure 32A shows Campath-1H Binding curves of ("C1H"), chimeric 2C3 antibody, and humanized 2C3-SFD1/K12 antibody to primary human T cells and huCD52 gene transgenic mouse T cells. Figure 32B shows Campath-1H Binding curves of ("C1H"), chimeric 9D9 antibody, and humanized 9D9 antibody to primary human T cells and huCD52 gene transgenic mouse T cells. Figure 32C shows Campath-1H Binding curves of ("C1H"), chimeric 12G6 antibody and humanized 12G6 antibody to primary human T cells and huCD52 gene transgenic mouse T cells.

第33圖為一種顯示Campath-1H、嵌合2C3及12G6抗體及人類化2C3及12G6抗體至表現人類及基因轉殖老鼠T細胞的huCD52之相對結合效率的表。Figure 33 shows a display of Campath-1H A table showing the relative binding efficiencies of chimeric 2C3 and 12G6 antibodies and humanized 2C3 and 12G6 antibodies to huCD52 expressing human and gene-transferred mouse T cells.

第34圖藉由流式細胞計數法說明人類化抗-CD52 Campath-1H、2C3、12G6、及9D9抗體至人類週邊血液單核細胞族群的經定義子集之相對結合形式。這些統計表顯示人類化抗-CD52抗體結合係相當於Campath-1H對各種表現CD52的人類PBMC子集的抗體結合。X軸表示由所結合抗-CD52抗體所放出的螢光,其中每一個峰的面積表示總細胞族群。Figure 34 illustrates the humanized anti-CD52 Campath-1H by flow cytometry The relative binding of the 2C3, 12G6, and 9D9 antibodies to a defined subset of human peripheral blood mononuclear cell populations. These statistics show that the humanized anti-CD52 antibody binding line is equivalent to Campath-1H Antibody binding to various human PBMC subsets that express CD52. The X-axis represents the fluorescence emitted by the bound anti-CD52 antibody, wherein the area of each peak represents the total cell population.

第35圖為顯示嵌合及人類化7F11抗體媒介相當ADCC活性於表現CD52的細胞的圖。Figure 35 is a graph showing that chimeric and humanized 7F11 antibody vectors are equivalent to ADCC activity in cells expressing CD52.

第36圖為顯示嵌合及人類化7F11抗體媒介CDC活性於表現CD52的細胞的圖。Figure 36 is a graph showing chimeric and humanized 7F11 antibody vector CDC activity in cells expressing CD52.

第37圖為顯示嵌合及人類化2C3抗體媒介ADCC活性於表現CD52的細胞的圖。Figure 37 is a diagram showing chimeric and humanized 2C3 antibody mediator ADCC activity in cells expressing CD52.

第38圖為顯示嵌合及人類化2C3抗體媒介CDC活性於表現CD52的細胞的圖。Figure 38 is a graph showing chimeric and humanized 2C3 antibody mediator CDC activity in cells expressing CD52.

第39圖為顯示嵌合及人類化12G6抗體媒介ADCC活性於表現CD52的細胞的圖。Figure 39 is a graph showing chimeric and humanized 12G6 antibody mediator ADCC activity in cells expressing CD52.

第40圖為顯示嵌合及人類化12G6抗體媒介CDC活性於表現CD52的細胞的圖。Figure 40 is a graph showing chimeric and humanized 12G6 antibody vector CDC activity in cells expressing CD52.

第41圖為顯示嵌合及人類化9D9抗體媒介ADCC活性於表現CD52的細胞的圖。Figure 41 is a graph showing that chimeric and humanized 9D9 antibody mediator ADCC activity is expressed in cells expressing CD52.

第42圖為顯示嵌合及人類化9D9抗體媒介CDC活性於表現CD52的細胞的圖。Figure 42 is a graph showing chimeric and humanized 9D9 antibody vector CDC activity in cells expressing CD52.

第43圖為一種顯示人類化抗-CD52抗體於初級T細胞的ADCC活性的圖。Figure 43 is a graph showing the ADCC activity of a humanized anti-CD52 antibody in primary T cells.

第44圖為一種顯示人類化抗-CD52抗體於初級T細胞的CDC活性的圖。Figure 44 is a graph showing the CDC activity of a humanized anti-CD52 antibody in primary T cells.

第45圖為一種顯示Campath-1H而非其他抗-CD52抗體的中性化的圖,其係使用包含抗-Campath-1H中和抗體的CAMMS223研究人類血清樣品。血清樣品係在第12個月(M12)及第13個月(M13)取自代表性病人(MS-1)。Figure 45 is a diagram showing the neutralization of Campath-1H but not other anti-CD52 antibodies using anti-Campath-1H Human serum samples were studied by neutralizing antibodies to CAMMS223. Serum samples were taken from representative patients (MS-1) at month 12 (M12) and 13 months (M13).

第46A-46E圖顯示在使用Campath-1H(「Campath」)及人類化4B10-H1/K1(「4B10」)抗體投藥之後72小時血液中CD4+ T細胞、CD8+ T細胞、B220+ B細胞、NK細胞、骨髓樣的細胞及嗜中性球的含量。Figure 46A-46E shows the use of Campath-1H ("Campath") and humanized 4B10-H1/K1 ("4B10") antibody 72 hours after administration of blood CD4+ T cells, CD8+ T cells, B220+ B cells, NK cells, bone marrow-like cells and neutrophils content.

第47A-47E圖顯示在使用Campath-1H(「Campath」)及人類化4B10-H1/K1(「4B10」)抗體投藥之後72小時脾臟中CD4+ T細胞、CD8+ T細胞、B220+ B細胞、NK細胞、骨髓樣的細胞、嗜中性球及巨噬細胞的含量。Figure 47A-47E shows the use of Campath-1H ("Campath") and humanized 4B10-H1/K1 ("4B10") antibody 72 hours after administration of CD4+ T cells, CD8+ T cells, B220+ B cells, NK cells, bone marrow-like cells, neutrophils and The content of macrophages.

第48A-48E圖顯示在使用Campath-1H(「Campath」)及人類化4B10-H1/K1(「4B10」)抗體投藥之後2小時循環細胞介素的含量。Figure 48A-48E shows the use of Campath-1H ("Campath") and the content of circulating interleukins 2 hours after administration of the humanized 4B10-H1/K1 ("4B10") antibody.

第49A及49B圖顯示在使用Campath-1H(「Campath」)及人類化4B10-H1/K1(「4B10」)抗體,(毫克/公斤)投藥之後循環細胞介素隨時間的再增殖。Figures 49A and 49B show the use of Campath-1H ("Campath") and humanized 4B10-H1/K1 ("4B10") antibody, (mg/kg) re-proliferation of circulating interleukins over time.

第50A-50E圖顯示在使用人類化7F11-SFD1/K2(「7F11 SFD1」)及7F11-SFD2/K2(「7F11 SFD2」)抗體投藥之後72小時血液中CD4+ T細胞、CD8+ T細胞、B220+ B細胞、NK細胞、骨髓樣的細胞及嗜中性球的含量。Figure 50A-50E shows CD4+ T cells, CD8+ T cells, B220+ B in the blood 72 hours after administration of humanized 7F11-SFD1/K2 ("7F11 SFD1") and 7F11-SFD2/K2 ("7F11 SFD2") antibodies. The content of cells, NK cells, bone marrow-like cells, and neutrophils.

第51A-51E圖顯示在使用人類化7F11-SFD1/K2(「7F11 SFD1」)及7F11-SFD2/K2(「7F11SFD2」)抗體投藥之後72小時脾臟中CD4+ T細胞、CD8+ T細胞、B220+ B細胞、NK細胞、骨髓樣的細胞及嗜中性球的含量。Figure 51A-51E shows CD4+ T cells, CD8+ T cells, B220+ B cells in the spleen 72 hours after administration of humanized 7F11-SFD1/K2 ("7F11 SFD1") and 7F11-SFD2/K2 ("7F11SFD2") antibodies. , NK cells, bone marrow-like cells and neutrophils.

第52A-52F圖顯示在使用人類化7F11-SFD1/K2(「7F11 SFD1」)及7F11-SFD2/K2(「7F11 SFD2」)抗體投藥之後2小時循環細胞介素的含量。Figures 52A-52F show the levels of circulating interleukins 2 hours after administration of humanized 7F11-SFD1/K2 ("7F11 SFD1") and 7F11-SFD2/K2 ("7F11 SFD2") antibodies.

第53A及53B圖顯示在使用人類化7F11-SFD1/K2(「7F11 SFD1」)及7F11-SFD2/K2(「7F11 SFD2」)抗體投藥,(毫克/公斤)之後循環細胞介素隨時間的再增殖。Figures 53A and 53B show the circulating interleukins over time after administration of humanized 7F11-SFD1/K2 ("7F11 SFD1") and 7F11-SFD2/K2 ("7F11 SFD2") antibodies, (mg/kg) proliferation.

第54A及54B圖顯示在使用Campath-1H(「Campath」)、7F11-嵌合抗體、及人類化7F11-SFD1/K2與7F11-SFD2/K2抗體投藥之後72小時血液中CD4+ T細胞、CD8+ T細胞及B220+ B細胞的含量。Figures 54A and 54B show the use of Campath-1H The content of CD4+ T cells, CD8+ T cells and B220+ B cells in the blood 72 hours after ("Campath"), 7F11-chimeric antibody, and humanized 7F11-SFD1/K2 and 7F11-SFD2/K2 antibodies were administered.

第55圖顯示投藥之後血液中Campath-1H(「Campath」)、7F11-c嵌合抗體及人類化7F11-SFD1/K2與7F11-SFD2/K2抗體隨時間的含量。Figure 55 shows Campath-1H in the blood after administration. ("Campath"), 7F11-c chimeric antibody and humanized 7F11-SFD1/K2 and 7F11-SFD2/K2 antibody content over time.

第56A-56E圖顯示使用2C3-SFD1/K12抗體投藥之後72小時血液中CD4+ T細胞、CD8+ T細胞、B220+ B細胞、NK細胞及嗜中性球的含量。Figures 56A-56E show the levels of CD4+ T cells, CD8+ T cells, B220+ B cells, NK cells, and neutrophils in the blood 72 hours after administration with the 2C3-SFD1/K12 antibody.

第57A-57E圖顯示使用2C3-SFD1/K12抗體投藥之後72小時脾臟中CD4+ T細胞、CD8+ T細胞、B220+ B細胞、NK細胞及嗜中性球的含量。Figures 57A-57E show the levels of CD4+ T cells, CD8+ T cells, B220+ B cells, NK cells, and neutrophils in the spleen 72 hours after administration with the 2C3-SFD1/K12 antibody.

第58A-58F圖顯示使用2C3-SFD1/K12("2C3")抗體投藥之後2小時循環細胞介素的含量。Figures 58A-58F show the amount of circulating interleukins 2 hours after administration with the 2C3-SFD1/K12 ("2C3") antibody.

第59圖顯示在使用2C3-SFD1/K12抗體投藥,(毫克/公斤)之後循環細胞介素隨時間的再增殖。Figure 59 shows the repopulation of circulating interleukins over time after administration with 2C3-SFD1/K12 antibody, (mg/kg).

第60A-60E圖顯示在使用12G6-SFD1/K11抗體投藥之後72小時血液中CD4+ T細胞、CD8+ T細胞、B220+ B細胞、NK細胞、骨髓樣的細胞、巨噬細胞及嗜中性球的含量。Figure 60A-60E shows the levels of CD4+ T cells, CD8+ T cells, B220+ B cells, NK cells, bone marrow-like cells, macrophages, and neutrophils in the blood 72 hours after administration with the 12G6-SFD1/K11 antibody. .

第61A-61E圖顯示在使用12G6-SFD1/K11抗體投藥之後72小時脾臟中CD4+ T細胞、CD8+ T細胞、B220+ B細胞、NK細胞、巨噬細胞、嗜中性球及骨髓樣的細胞的含量。Figure 61A-61E shows the content of CD4+ T cells, CD8+ T cells, B220+ B cells, NK cells, macrophages, neutrophils and myeloid cells in the spleen 72 hours after administration with the 12G6-SFD1/K11 antibody. .

第62A-62F圖顯示在使用12G6-SFD1/K11(「12G6 hu」)抗體投藥之後2小時循環細胞介素的含量。Panels 62A-62F show circulating interleukin levels 2 hours after administration with 12G6-SFD1/K11 ("12G6 hu") antibody.

第63圖顯示在使用12G6-SFD1/K11抗體投藥,(毫克/公斤)之後循環淋巴細胞隨時間的再增殖。Figure 63 shows repopulation of circulating lymphocytes over time following administration of 12G6-SFD1/K11 antibody, (mg/kg).

第64A-64C圖顯示投藥之後血液中2C3-嵌合、2C3-SFD1/K12、12G6-嵌合、12G6-SFD1/K11、9D9-嵌合及9D9-H10/K12抗體隨時間的含量。Figure 64A-64C shows the levels of 2C3-chimeric, 2C3-SFD1/K12, 12G6-chimeric, 12G6-SFD1/K11, 9D9-chimeric and 9D9-H10/K12 antibodies in the blood after administration.

第65A-65E圖顯示在使用9D9-H10/K12(「9D9」)抗體投藥之後72小時血液中CD4+ T細胞、CD8+ T細胞、B220+ B細胞、NK細胞、骨髓樣的細胞、巨噬細胞及嗜中性球的含量。Figure 65A-65E shows CD4+ T cells, CD8+ T cells, B220+ B cells, NK cells, bone marrow-like cells, macrophages and hobbies in the blood 72 hours after administration with 9D9-H10/K12 ("9D9") antibody. The content of the neutral ball.

第66A-66E圖顯示在使用9D9-H10/K12(「9D9」)抗體投藥之後72小時脾臟中CD4+ T細胞、CD8+ T細胞、B220+ B細胞、NK細胞、骨髓樣的細胞、嗜中性球及巨噬細胞的含量。Figure 66A-66E shows CD4+ T cells, CD8+ T cells, B220+ B cells, NK cells, bone marrow-like cells, neutrophils and spleens in the spleen 72 hours after administration with 9D9-H10/K12 ("9D9") antibody. The content of macrophages.

第67A-67F圖顯示在使用9D9-H10/K12(「9D9」)抗體投藥之後2小時循環細胞介素的含量。Figures 67A-67F show the amount of circulating interleukins 2 hours after administration of the 9D9-H10/K12 ("9D9") antibody.

第68圖顯示在使用9D9-H10/K12(「9D9」)抗體,(毫克/公斤)投藥之後循環淋巴細胞隨時間的再增殖。Figure 68 shows repopulation of circulating lymphocytes over time following administration of 9D9-H10/K12 ("9D9") antibody, (mg/kg).

第69A-69D圖顯示在使用Campath-1H(「Campath」)、2C3-SFD1/K12(「2C3」)、12G6-SFD1/K11(「12G6」)及9D9-H10/K12(「9D9」)抗體投藥之後72小時血液中整體淋巴細胞族群(CD4+ T細胞、CD8+ T細胞、及B細胞)及CD4+ T細胞、CD8+ T細胞、B220+ B細胞及NK細胞子形式的含量。Figure 69A-69D shows the use of Campath-1H ("Campath"), 2C3-SFD1/K12 ("2C3"), 12G6-SFD1/K11 ("12G6"), and 9D9-H10/K12 ("9D9") antibodies were administered to the whole lymphocyte population at 72 hours after administration ( The content of CD4+ T cells, CD8+ T cells, and B cells) and CD4+ T cells, CD8+ T cells, B220+ B cells, and NK cell forms.

第70A-70D圖顯示在使用Campath-1H(「Campath」)、2C3-SFD1/K12(「2C3」)、12G6-SFD1/K11(「12G6」)、及9D9-H10/K12(「9D9」)抗體投藥之後72小時脾臟中整體淋巴細胞族群(CD4+ T細胞、CD8+ T細胞、及B細胞)及CD4+ T細胞、CD8+ T細胞、B220+ B細胞及NK細胞子形式的含量。Figure 70A-70D shows the use of Campath-1H ("Campath"), 2C3-SFD1/K12 ("2C3"), 12G6-SFD1/K11 ("12G6"), and 9D9-H10/K12 ("9D9") antibody 72 hours after administration of the whole lymphocyte population in the spleen (CD4+ T cells, CD8+ T cells, and B cells) and CD4+ T cells, CD8+ T cells, B220+ B cells, and NK cell forms.

第71A-71F圖顯示在使用Campath-1H、2C3-SFD1/K12、12G6-SFD1/K11、及9D9-H10/K12抗體投藥之後2小時循環細胞介素的含量。Figure 71A-71F shows the use of Campath-1H The content of interleukins was 2 hours after administration of 2C3-SFD1/K12, 12G6-SFD1/K11, and 9D9-H10/K12 antibodies.

第72圖顯示在使用9D9-H10/K12及9D9-H11/K12抗體投藥之後72小時血液中CD4+ T細胞、CD8+ T細胞、B220+ B細胞及NK細胞的含量。Figure 72 shows the levels of CD4+ T cells, CD8+ T cells, B220+ B cells, and NK cells in the blood 72 hours after administration with the 9D9-H10/K12 and 9D9-H11/K12 antibodies.

第73圖顯示在使用9D9-H10/K12及9D9-H11/K12抗體投藥之後72小時脾臟中CD4+ T細胞、CD8+ T細胞、B220+ B細胞及NK細胞的含量。Figure 73 shows the contents of CD4+ T cells, CD8+ T cells, B220+ B cells, and NK cells in the spleen 72 hours after administration with the 9D9-H10/K12 and 9D9-H11/K12 antibodies.

第74A-74D圖顯示在使用12G6-SFD1/K11(「12G6 K11」)及12G6-SFD1/K12(「12G6 K12」)抗體投藥之後72小時血液中CD4+ T細胞、CD8+ T細胞、B220+ B細胞、NK細胞及骨髓樣的細胞的含量。Figure 74A-74D shows CD4+ T cells, CD8+ T cells, B220+ B cells in the blood 72 hours after administration of 12G6-SFD1/K11 ("12G6 K11") and 12G6-SFD1/K12 ("12G6 K12") antibodies. The content of NK cells and bone marrow-like cells.

第75A-75D圖顯示在使用12G6-SFD1/K11(「12G6 K11」)及12G6-SFD1/K12(「12G6 K12」)抗體投藥之後72小時脾臟中CD4+ T細胞、CD8+ T細胞、B220+ B細胞、NK細胞及骨髓樣的細胞的含量。Figure 75A-75D shows CD4+ T cells, CD8+ T cells, B220+ B cells in the spleen 72 hours after administration with 12G6-SFD1/K11 ("12G6 K11") and 12G6-SFD1/K12 ("12G6 K12") antibodies, The content of NK cells and bone marrow-like cells.

第76圖顯示在使用9D9-H11/K12、9D9-H16/K13及9D9-H18/K13抗體投藥之後72小時血液中整體淋巴細胞族群(CD4+ T細胞、CD8+ T細胞及B220+ B細胞)的含量。Figure 76 shows the content of the whole lymphocyte population (CD4+ T cells, CD8+ T cells and B220+ B cells) in the blood 72 hours after administration with the 9D9-H11/K12, 9D9-H16/K13 and 9D9-H18/K13 antibodies.

第77A-77D圖顯示在使用9D9-H11/K12、9D9-H16/K13及9D9-H18/K13抗體投藥之後72小時血液中CD4+ T細胞、CD8+ T細胞、B220+ B細胞、NK細胞及骨髓樣的細胞子形式的含量。Figure 77A-77D shows CD4+ T cells, CD8+ T cells, B220+ B cells, NK cells, and bone marrow in the blood 72 hours after administration with 9D9-H11/K12, 9D9-H16/K13, and 9D9-H18/K13 antibodies. The content of the cell subform.

第78圖顯示在使用9D9-H11/K12、9D9-H16/K13及9D9-H18/K13抗體投藥之後72小時脾臟中整體淋巴細胞族群(CD4+ T細胞、CD8+ T細胞及B220+ B細胞)的含量。Figure 78 shows the content of the whole lymphocyte population (CD4+ T cells, CD8+ T cells and B220+ B cells) in the spleen 72 hours after administration with the 9D9-H11/K12, 9D9-H16/K13 and 9D9-H18/K13 antibodies.

第79A-79D圖顯示在使用9D9-H11/K12、9D9-H16/K13及9D9-H18/K13抗體投藥之後72小時脾臟中CD4+ T細胞、CD8+ T細胞、B220+ B細胞、NK細胞及骨髓樣的細胞子形式的含量。Figure 79A-79D shows CD4+ T cells, CD8+ T cells, B220+ B cells, NK cells, and bone marrow-like cells in the spleen 72 hours after administration with 9D9-H11/K12, 9D9-H16/K13, and 9D9-H18/K13 antibodies. The content of the cell subform.

第80A-80F圖顯示在使用9D9-H11/K12、9D9-H16/K13及9D9-H18/K13抗體投藥之後2小時循環細胞介素的含量。Panels 80A-80F show circulating interleukin levels 2 hours after administration with 9D9-H11/K12, 9D9-H16/K13 and 9D9-H18/K13 antibodies.

第81A及81B圖顯示投藥之後血液中2C3-SFD1/K12、12G6-SFD1/K11、12G6-SFD1/K12、9D9-H16/K13及9D9-H18/K13抗體隨時間的含量。Figures 81A and 81B show the levels of 2C3-SFD1/K12, 12G6-SFD1/K11, 12G6-SFD1/K12, 9D9-H16/K13, and 9D9-H18/K13 antibodies in the blood after administration.

第82A-82F圖顯示在使用Campath-1H(「Campath」)、2C3-SFD1/K11、12G6-SFD1/K11、12G6-SFD1/K12、9D9-H16/K13或9D9-H18/K13抗體投藥之後隨48-小時時間期間血液中細胞介素的含量。Figure 82A-82F shows the use of Campath-1H ("Campath"), 2C3-SFD1/K11, 12G6-SFD1/K11, 12G6-SFD1/K12, 9D9-H16/K13 or 9D9-H18/K13 antibodies administered with interleukins in the blood during 48-hour period content.

第83A-83E圖顯示在使用Campath-1H(「Campath」)、2C3-SFD1/K11、12G6-SFD1/K11、12G6-SFD1/K12、9D9-H16/K13或9D9-H18/K13抗體投藥之後72小時脾臟中整體淋巴細胞、CD4+ T細胞、CD8+ T細胞、B220+ B細胞、NK細胞及骨髓樣的細胞的含量。Figure 83A-83E shows the use of Campath-1H ("Campath"), 2C3-SFD1/K11, 12G6-SFD1/K11, 12G6-SFD1/K12, 9D9-H16/K13 or 9D9-H18/K13 antibody, 72 hours after administration of whole lymphocytes, CD4+ T cells, The content of CD8+ T cells, B220+ B cells, NK cells and bone marrow-like cells.

第84A-84G圖顯示在使用Campath-1H(「Campath」)、2C3-SFD1/K12、9D9-H16/K13及12G6-SFD1/K12抗體投藥之後循環CD4+與CD8+ T細胞、調節T細胞、B細胞、NK細胞、嗜中性球及巨噬細胞隨時間的再增殖。Figure 84A-84G shows the use of Campath-1H ("Campath"), 2C3-SFD1/K12, 9D9-H16/K13 and 12G6-SFD1/K12 antibodies circulate CD4+ and CD8+ T cells, regulate T cells, B cells, NK cells, neutrophils and macrophages The cells repopulate over time.

第85圖顯示FITC-標記Campath-1H("Campath")、2C3-SFD1/K12("2C3 K12")、12G6-SFD1/K11("12G6 K11")、12G6-SFD1/K12("12G6 K12")、9D9-H16/K13("9D9 H16")、及9D9-H18/K13("9D9 H18")抗體特定地結合至脾臟中huCD52淋巴細胞族群之能力。Figure 85 shows FITC-labeled Campath-1H ("Campath"), 2C3-SFD1/K12 ("2C3 K12"), 12G6-SFD1/K11 ("12G6 K11"), 12G6-SFD1/K12 ("12G6 K12"), 9D9-H16/K13 ("9D9 The ability of H16"), and 9D9-H18/K13 ("9D9 H18") antibodies to specifically bind to the huCD52 lymphocyte population in the spleen.

第86A-86E圖顯示在使用Campath-1H(「Campath」)、2C3-SFD1/K12、12G6-SFD1/K11、12G6-SFD1/K12、9D9-H16/K13、及9D9-H18/K13抗體投藥之後72小時血液中整體淋巴細胞族群(CD4+ T細胞、CD8+ T細胞及B220+ B細胞)及CD4+ T細胞、CD8+ T細胞、B220+ B細胞、NK細胞及骨髓樣的細胞子形式的含量。Figure 86A-86E shows the use of Campath-1H ("Campath"), 2C3-SFD1/K12, 12G6-SFD1/K11, 12G6-SFD1/K12, 9D9-H16/K13, and 9D9-H18/K13 antibodies, 72 hours after administration of the whole lymphocyte population (CD4+ T The content of cells, CD8+ T cells and B220+ B cells) and CD4+ T cells, CD8+ T cells, B220+ B cells, NK cells and bone marrow-like cell forms.

第87A-87E圖顯示在使用Campath-1H(「Campath」)、2C3-SFD1/K12、12G6-SFD1/K11、12G6-SFD1/K12、9D9-H16/K13及9D9-H18/K13抗體投藥之後72小時脾臟中整體淋巴細胞族群(CD4+ T細胞、CD8+ T細胞及B220+ B細胞)及CD4+ T細胞、CD8+ T細胞、B220+ B細胞、NK細胞及骨髓樣的細胞子形式的含量。Figure 87A-87E shows the use of Campath-1H ("Campath"), 2C3-SFD1/K12, 12G6-SFD1/K11, 12G6-SFD1/K12, 9D9-H16/K13 and 9D9-H18/K13 antibodies were administered to the spleen in the whole lymphocyte population (CD4+ T cells) 72 hours after administration , CD8+ T cells and B220+ B cells) and CD4+ T cells, CD8+ T cells, B220+ B cells, NK cells and bone marrow-like cell forms.

第88A-88F圖顯示在使用Campath-1H(「Campath」)、2C3-SFD1/K12、12G6-SFD1/K11、12G6-SFD1/K12、9D9-H16/K13及9D9-H18/K13抗體投藥之後2小時循環細胞介素的含量。Figure 88A-88F shows the use of Campath-1H ("Campath"), 2C3-SFD1/K12, 12G6-SFD1/K11, 12G6-SFD1/K12, 9D9-H16/K13, and 9D9-H18/K13 antibody circulating interleukin content 2 hours after administration.

第89A-89D圖顯示在使用Campath-1H(「Campath」)、2C3-SFD1/K12、9D9-H16/K13及12G6-SFD1/K12抗體投藥之後72小時血液中CD4+ T細胞、CD8+ T細胞、B220+ B細胞、及NK/骨髓樣的細胞子形式的含量。Figure 89A-89D shows the use of Campath-1H ("Campath"), 2C3-SFD1/K12, 9D9-H16/K13, and 12G6-SFD1/K12 antibodies in the blood 72 hours after administration of CD4+ T cells, CD8+ T cells, B220+ B cells, and NK/myeloid-like cells The content of the form.

第90A-90D圖顯示在使用Campath-1H(「Campath」)、2C3-SFD1/K12、9D9-H16/K13及12G6-SFD1/K12抗體投藥之後72小時脾臟中CD4+ T細胞、CD8+ T細胞、B220+ B細胞、及NK/骨髓樣的細胞子形式的含量。Figure 90A-90D shows the use of Campath-1H CD4+ T cells, CD8+ T cells, B220+ B cells, and NK/myeloid-like cells in the spleen 72 hours after administration of ("Campath"), 2C3-SFD1/K12, 9D9-H16/K13, and 12G6-SFD1/K12 antibodies The content of the form.

第91A-91D圖顯示在使用Campath-1H(「Campath」)、2C3-SFD1/K12、9D9-H16/K13及12G6-SFD1/K12抗體投藥之後72小時淋巴結中CD4+ T細胞、CD8+ T細胞、B220+ B細胞、及NK/骨髓樣的細胞子形式的含量。Figure 91A-91D shows the use of Campath-1H ("Campath"), 2C3-SFD1/K12, 9D9-H16/K13, and 12G6-SFD1/K12 antibody CD4+ T cells, CD8+ T cells, B220+ B cells, and NK/myeloid-like cells in the lymph nodes 72 hours after administration The content of the form.

第92A圖顯示huCD52-KI/KO及非-基因轉殖對照老鼠中於CD4+ T細胞、CD8+ T細胞、B220+ B細胞、及NK/骨髓樣的細胞子形式的huCD52表現位準。第92B圖顯示huCD52-KI/KO及huCD52CD1基因轉殖老鼠中於CD4+ T細胞、CD8+ T細胞、及B細胞的huCD52表現位準。Figure 92A shows the level of huCD52 expression in CD4+ T cells, CD8+ T cells, B220+ B cells, and NK/myeloid cell subforms in huCD52-KI/KO and non-gene transgenic control mice. Figure 92B shows the huCD52 expression levels of CD4+ T cells, CD8+ T cells, and B cells in huCD52-KI/KO and huCD52CD1 gene transgenic mice.

第93圖顯示與Campath-1H對照組相較來自各種製造來源("小規模"及"大規模")的12G6-SFD1/K12與2C3-SFD1/K12抗體的huCD52之結合。Figure 93 shows with Campath-1H The control group was compared to huCD52 of 12G6-SFD1/K12 and 2C3-SFD1/K12 antibodies from various manufacturing sources ("small scale" and "large scale").

第94圖顯示在使用來自各種製造來源("小規模"及"大規模")的12G6-SFD1/K12及2C3-SFD1/K12抗體投藥之後72小時血液中整體淋巴細胞族群(CD4+ T細胞、CD8+ T細胞、B220+ B細胞及NK細胞)的含量。Figure 94 shows the overall lymphocyte population (CD4+ T cells, CD8+) in the blood 72 hours after administration of 12G6-SFD1/K12 and 2C3-SFD1/K12 antibodies from various manufacturing sources ("small scale" and "large scale"). The content of T cells, B220+ B cells and NK cells).

第95圖顯示在投藥之後血液中2C3-SFD1/K12、9D9-H16/K13及12G6-SFD1/K12抗體隨時間的含量。Figure 95 shows the content of 2C3-SFD1/K12, 9D9-H16/K13 and 12G6-SFD1/K12 antibodies in the blood over time after administration.

第96圖證明隨疾病惡化時間2C3-SFD1/K12及12G6-SFD1/K12的EAE臨床評分。Figure 96 demonstrates the EAE clinical scores for 2C3-SFD1/K12 and 12G6-SFD1/K12 with disease progression time.

第97A及97B圖證明Campath1H(「Campath」)、2C3-SFD1/K12(「2C3」)、His435Ala 2C3-SFD1/K12(「H435A 2C3」)及His310Ala/His435Gln 2C3-SFD1/K12(「H310A/H435Q2C3」)結合至老鼠及人類FcRn分子之能力。Figures 97A and 97B demonstrate Campath1H ("Campath"), 2C3-SFD1/K12 ("2C3"), His435Ala 2C3-SFD1/K12 ("H435A 2C3"), and His310Ala/His435Gln 2C3-SFD1/K12 ("H310A/H435Q2C3") bind to mice and humans The ability of the FcRn molecule.

第98圖顯示在非基因轉殖老鼠中2C3-SFD1/K12(「2C3未修飾」)、2C3-SFD1/K12-修飾1(「2C3-Fc突變體1」)及2C3-SFD1/K12-修飾2(「2C3-Fc突變體2」)的本體內清除作用。Figure 98 shows 2C3-SFD1/K12 ("2C3 unmodified"), 2C3-SFD1/K12-modified 1 ("2C3-Fc mutant 1") and 2C3-SFD1/K12-modification in non-gene-transferred mice 2 ("2C3-Fc mutant 2") in vivo clearance.

第99圖顯示在huCD52基因轉殖老鼠中2C3-SFD1/K12(「2C3」)、2C3-SFD1/K12-修飾1(「2C3-Fc突變體1」)及2C3-SFD1/K12-修飾2(「2C3-Fc突變體2」)的本體內清除作用。Figure 99 shows 2C3-SFD1/K12 ("2C3"), 2C3-SFD1/K12-modification 1 ("2C3-Fc mutant 1") and 2C3-SFD1/K12-modification 2 in huCD52 gene-transferred mice ( The in vivo clearance of "2C3-Fc mutant 2").

第100A及100B圖顯示在使用2C3-SFD1/K12(「2C3」)、2C3-SFD1/K12-修飾1(「2C3-Fc突變體1」)及2C3-SFD1/K12-修飾2(「2C3-Fc突變體2」)抗體投藥之後72小時血液及脾臟中整體淋巴細胞族群(CD4+ T細胞、CD8+ T細胞、B220+ B細胞及NK細胞)的含量。Figures 100A and 100B show the use of 2C3-SFD1/K12 ("2C3"), 2C3-SFD1/K12-modification 1 ("2C3-Fc mutant 1") and 2C3-SFD1/K12-modification 2 ("2C3- Fc mutant 2") The content of the whole lymphocyte population (CD4+ T cells, CD8+ T cells, B220+ B cells, and NK cells) in the blood and spleen 72 hours after administration of the antibody.

第101A及101B圖為Biacore T100試驗的代表性感應圖譜以決定人類化12G6-SFD1/K12抗體及由丙胺酸掃描產生的突變肽的抗原決定區特異性。第101A圖顯示在12G6-SFD1/K12及MUT 8肽之間沒有任何結合,且第101B圖顯示在12G6-SFD1/K12及MUT 9肽之間存在結合。Figures 101A and 101B are representative induction profiles of the Biacore T100 assay to determine the epitope-specificity of the humanized 12G6-SFD1/K12 antibody and the mutant peptide produced by alanine scanning. Figure 101A shows no binding between the 12G6-SFD1/K12 and MUT 8 peptides, and Figure 101B shows the presence of binding between the 12G6-SFD1/K12 and MUT 9 peptides.

第102圖顯示授予體BMS486的TCR Vβ分析。使用Campath-1H肽族群986-989教育的CD4+ T細胞顯現單一Vβ(Vβ3)的優先膨脹。Figure 102 shows the TCR Vβ analysis of the donor BMS486. Use Campath-1H The CD4+ T cells educated by the peptide population 986-989 exhibit preferential expansion of a single Vβ (Vβ3).

第103圖顯示授予體BMS928的TCR Vβ分析。使用12G6-SFD1/K12肽族群1066-67-68及1083-84-85教育的CD4+ T細胞顯現單一Vβ(Vβ20)的優先膨脹。Figure 103 shows the TCR Vβ analysis of the donor BMS928. The preferential expansion of a single Vβ (Vβ20) was visualized using CD4+ T cells educated by 12G6-SFD1/K12 peptide populations 1066-67-68 and 1083-84-85.

第104A-104J圖顯示Campath-1H致免疫性評估。增生反應示於個別授予體A-J的CPM。X軸說明用於刺激自體移植CD4+ T細胞三次的肽族群。每一組T細胞使用以教育抗原/肽族群脈衝的自體移植DC(特異性反應,左邊條狀物,白色)、不相關的DR結合肽(中間條狀物,細條)、或是介質(右邊條狀物,黑色)重複分析三次。Figure 104A-104J shows Campath-1H Immunogenicity assessment. The proliferative response is shown in the CPM of the individual donor AJ. The X-axis illustrates the peptide population used to stimulate autologous transplantation of CD4+ T cells three times. Each group of T cells uses autologous transplanted DCs (specific reactions, left bars, white), unrelated DR-binding peptides (intermediate strips, thin strips), or media (s) that are pulsed with educational antigen/peptide populations. The strip on the right, black) was analyzed three times.

第105A-105J圖顯示12G6-SFD1/K12致免疫性評估。增生反應示於個別授予體A-J的CPM。X軸說明用於刺激自體移植CD4+ T細胞三次的肽族群。每一組T細胞使用以教育肽族群脈衝的自體移植DC(特異性反應,左邊條狀物,白色)、不相關的DR結合肽(中間條狀物,細條)、或是介質(右邊條狀物,黑色)重複分析三次。在沒有介質控制試驗的族群中,左邊條狀物(白色)表示以教育肽脈衝的DC,及右邊條狀物(細條)表示以不相關肽脈衝的DC。Figures 105A-105J show 12G6-SFD1/K12 immunogenicity assessment. The proliferative response is shown in the CPM of the individual donor A-J. The X-axis illustrates the peptide population used to stimulate autologous transplantation of CD4+ T cells three times. Each group of T cells uses autologous transplantation DC (specific reaction, left strip, white) pulsed with educational peptide population, unrelated DR binding peptide (intermediate strip, thin strip), or medium (right strip) (black, repeated) three times. In the population without media control experiments, the left bar (white) represents the DC pulsed with the educational peptide, and the right bar (strip) represents the DC pulsed with the unrelated peptide.

第106圖顯示2C3-SFD1(SEQ ID NO: 272)的全長度人類化重鏈胺基酸序列及2C3-K12(SEQ ID NO: 273)的全長度人類化輕鏈胺基酸序列。信號序列以粗體及斜體表示及CDR加底線。Figure 106 shows the full length humanized heavy chain amino acid sequence of 2C3-SFD1 (SEQ ID NO: 272) and the full length humanized light chain amino acid sequence of 2C3-K12 (SEQ ID NO: 273). The signal sequence is shown in bold and italic and the CDR is underlined.

第107圖顯示7F11-SFD1(SEQ ID NO: 274)的全長度人類化重鏈胺基酸序列及7F11-K2(SEQ ID NO: 275)的全長度人類化輕鏈胺基酸序列。信號序列以粗體及斜體表示及CDR加底線。Figure 107 shows the full length humanized heavy chain amino acid sequence of 7F11-SFD1 (SEQ ID NO: 274) and the full length humanized light chain amino acid sequence of 7F11-K2 (SEQ ID NO: 275). The signal sequence is shown in bold and italic and the CDR is underlined.

第108圖顯示9D9-H16(SEQ ID NO: 276)及9D9-H18(SEQ ID NO: 277)的全長度人類化重鏈胺基酸序列,及9D9-K13(SEQ ID NO: 278)的全長度人類化輕鏈胺基酸序列。信號序列以粗體及斜體表示及CDR加底線。Figure 108 shows the full length humanized heavy chain amino acid sequence of 9D9-H16 (SEQ ID NO: 276) and 9D9-H18 (SEQ ID NO: 277), and the full length of 9D9-K13 (SEQ ID NO: 278) Humanized light chain amino acid sequence. The signal sequence is shown in bold and italic and the CDR is underlined.

第109圖顯示12G6-SFD1(SEQ ID NO: 279)的全長度人類化重鏈胺基酸序列及12G6-K12(SEQ ID NO: 280)的全長度人類化輕鏈胺基酸序列。信號序列以粗體及斜體表示及CDR加底線。Figure 109 shows the full length humanized heavy chain amino acid sequence of 12G6-SFD1 (SEQ ID NO: 279) and the full length humanized light chain amino acid sequence of 12G6-K12 (SEQ ID NO: 280). The signal sequence is shown in bold and italic and the CDR is underlined.

第110圖顯示4B10-H1(SEQ ID NO: 281)的全長度人類化重鏈胺基酸序列及4B10-K1(SEQ ID NO: 282)的全長度人類化輕鏈胺基酸序列。信號序列以粗體及斜體表示及CDR加底線。Figure 110 shows the full length humanized heavy chain amino acid sequence of 4B10-H1 (SEQ ID NO: 281) and the full length humanized light chain amino acid sequence of 4B10-K1 (SEQ ID NO: 282). The signal sequence is shown in bold and italic and the CDR is underlined.

第111圖顯示2C3-SFD1(SEQ ID NO: 283)的全長度人類化重鏈核酸序列及2C3-K12(SEQ ID NO: 284)的全長度人類化輕鏈核酸序列。信號序列加底線,變異區為粗體,及固定區為斜體。Figure 111 shows the full length humanized heavy chain nucleic acid sequence of 2C3-SFD1 (SEQ ID NO: 283) and the full length humanized light chain nucleic acid sequence of 2C3-K12 (SEQ ID NO: 284). The signal sequence is bottomed, the variation area is bold, and the fixed area is italic.

第112圖顯示7F11-SFD1(SEQ ID NO: 285)的全長度人類化重鏈核酸序列及7F11-K2(SEQ ID NO: 286)的全長度人類化輕鏈核酸序列。信號序列加底線,變異區為粗體,及固定區為斜體。Figure 112 shows the full length humanized heavy chain nucleic acid sequence of 7F11-SFD1 (SEQ ID NO: 285) and the full length humanized light chain nucleic acid sequence of 7F11-K2 (SEQ ID NO: 286). The signal sequence is bottomed, the variation area is bold, and the fixed area is italic.

第113圖顯示9D9-H16(SEQ ID NO: 287)及9D9-H18(SEQ ID NO: 288)的全長度人類化重鏈核酸序列。信號序列加底線,變異區為粗體,及固定區為斜體。Figure 113 shows full length humanized heavy chain nucleic acid sequences of 9D9-H16 (SEQ ID NO: 287) and 9D9-H18 (SEQ ID NO: 288). The signal sequence is bottomed, the variation area is bold, and the fixed area is italic.

第114圖顯示9D9-K13(SEQ ID NO: 289)的全長度人類化輕鏈核酸序列。信號序列加底線,變異區為粗體,及固定區為斜體。Figure 114 shows the full length humanized light chain nucleic acid sequence of 9D9-K13 (SEQ ID NO: 289). The signal sequence is bottomed, the variation area is bold, and the fixed area is italic.

第115圖顯示12G6-SFD1(SEQ ID NO: 290)的全長度人類化重鏈核酸序列及12G6-K12(SEQ ID NO: 291)的全長度人類化輕鏈核酸序列。信號序列加底線,變異區為粗體,及固定區為斜體。Figure 115 shows the full length humanized heavy chain nucleic acid sequence of 12G6-SFD1 (SEQ ID NO: 290) and the full length humanized light chain nucleic acid sequence of 12G6-K12 (SEQ ID NO: 291). The signal sequence is bottomed, the variation area is bold, and the fixed area is italic.

第116圖顯示4B10-H1(SEQ ID NO: 292)的全長度人類化重鏈核酸序列及4B10-K1(SEQ ID NO: 293)的全長度人類化輕鏈核酸序列。信號序列加底線,變異區為粗體,及固定區為斜體。Figure 116 shows the full length humanized heavy chain nucleic acid sequence of 4B10-H1 (SEQ ID NO: 292) and the full length humanized light chain nucleic acid sequence of 4B10-K1 (SEQ ID NO: 293). The signal sequence is bottomed, the variation area is bold, and the fixed area is italic.

<110> 建新公司 <110> Jianxin Company

<120> 抗人類CD52免疫球蛋白 <120> Anti-human CD52 immunoglobulin

<130> 001662-0029-WO1 <130> 001662-0029-WO1

<140> PCT/US2010/034704 <140> PCT/US2010/034704

<141> 2010-05-13 <141> 2010-05-13

<150> 61/177,837 <150> 61/177,837

<151> 2009-05-13 <151> 2009-05-13

<160> 294 <160> 294

<170> 版本3.5 <170> Version 3.5

<210> 1 <210> 1

<211> 107 <211> 107

<212> PRT <212> PRT

<213> 大鼠類 <213> Rats

<400> 1 <400> 1

<210> 2 <210> 2

<211> 112 <211> 112

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 2 <400> 2

<210> 3 <210> 3

<211> 112 <211> 112

<212> PRT <212> PRT

<213> 小鼠類 <213> Mouse

<400> 3 <400> 3

<210> 4 <210> 4

<211> 112 <211> 112

<212> PRT <212> PRT

<213> 小鼠類 <213> Mouse

<400> 4 <400> 4

<210> 5 <210> 5

<211> 112 <211> 112

<212> PRT <212> PRT

<213> 小鼠類 <213> Mouse

<400> 5 <400> 5

<210> 6 <210> 6

<211> 112 <211> 112

<212> PRT <212> PRT

<213> 小鼠類 <213> Mouse

<400> 6 <400> 6

<210> 7 <210> 7

<211> 112 <211> 112

<212> PRT <212> PRT

<213> 小鼠類 <213> Mouse

<400> 7 <400> 7

<210> 8 <210> 8

<211> 112 <211> 112

<212> PRT <212> PRT

<213> 小鼠類 <213> Mouse

<400> 8 <400> 8

<210> 9 <210> 9

<211> 111 <211> 111

<212> PRT <212> PRT

<213> 小鼠類 <213> Mouse

<400> 9 <400> 9

<210> 10 <210> 10

<211> 111 <211> 111

<212> PRT <212> PRT

<213> 小鼠類 <213> Mouse

<400> 10 <400> 10

<210> 11 <210> 11

<211> 111 <211> 111

<212> PRT <212> PRT

<213> 小鼠類 <213> Mouse

<400> 11 <400> 11

<210> 12 <210> 12

<211> 112 <211> 112

<212> PRT <212> PRT

<213> 小鼠類 <213> Mouse

<400> 12 <400> 12

<210> 13 <210> 13

<211> 113 <211> 113

<212> PRT <212> PRT

<213> 小鼠類 <213> Mouse

<400> 13 <400> 13

<210> 14 <210> 14

<211> 121 <211> 121

<212> PRT <212> PRT

<213> 大鼠類 <213> Rats

<400> 14 <400> 14

<210> 15 <210> 15

<211> 114 <211> 114

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 15 <400> 15

<210> 16 <210> 16

<211> 114 <211> 114

<212> PRT <212> PRT

<213> 小鼠類 <213> Mouse

<400> 16 <400> 16

<210> 17 <210> 17

<211> 114 <211> 114

<212> PRT <212> PRT

<213> 小鼠類 <213> Mouse

<400> 17 <400> 17

<210> 18 <210> 18

<211> 114 <211> 114

<212> PRT <212> PRT

<213> 小鼠類 <213> Mouse

<400> 18 <400> 18

<210> 19 <210> 19

<211> 114 <211> 114

<212> PRT <212> PRT

<213> 小鼠類 <213> Mouse

<400> 19 <400> 19

<210> 20 <210> 20

<211> 114 <211> 114

<212> PRT <212> PRT

<213> 小鼠類 <213> Mouse

<400> 20 <400> 20

<210> 21 <210> 21

<211> 114 <211> 114

<212> PRT <212> PRT

<213> 小鼠類 <213> Mouse

<400> 21 <400> 21

<210> 22 <210> 22

<211> 114 <211> 114

<212> PRT <212> PRT

<213> 小鼠類 <213> Mouse

<400> 22 <400> 22

<210> 23 <210> 23

<211> 114 <211> 114

<212> PRT <212> PRT

<213> 小鼠類 <213> Mouse

<400> 23 <400> 23

<210> 24 <210> 24

<211> 114 <211> 114

<212> PRT <212> PRT

<213> 小鼠類 <213> Mouse

<400> 24 <400> 24

<210> 25 <210> 25

<211> 117 <211> 117

<212> PRT <212> PRT

<213> 小鼠類 <213> Mouse

<400> 25 <400> 25

<210> 26 <210> 26

<211> 117 <211> 117

<212> PRT <212> PRT

<213> 小鼠類 <213> Mouse

<400> 26 <400> 26

<210> 27 <210> 27

<211> 11 <211> 11

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 27 <400> 27

<210> 28 <210> 28

<211> 16 <211> 16

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 28 <400> 28

<210> 29 <210> 29

<211> 16 <211> 16

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 29 <400> 29

<210> 30 <210> 30

<211> 16 <211> 16

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 30 <400> 30

<210> 31 <210> 31

<211> 16 <211> 16

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 31 <400> 31

<210> 32 <210> 32

<211> 16 <211> 16

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 32 <400> 32

<210> 33 <210> 33

<211> 16 <211> 16

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 33 <400> 33

<210> 34 <210> 34

<211> 7 <211> 7

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 34 <400> 34

<210> 35 <210> 35

<211> 7 <211> 7

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 35 <400> 35

<210> 36 <210> 36

<211> 7 <211> 7

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 36 <400> 36

<210> 37 <210> 37

<211> 7 <211> 7

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 37 <400> 37

<210> 38 <210> 38

<211> 7 <211> 7

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 38 <400> 38

<210> 39 <210> 39

<211> 7 <211> 7

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 39 <400> 39

<210> 40 <210> 40

<211> 7 <211> 7

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 40 <400> 40

<210> 41 <210> 41

<211> 7 <211> 7

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 41 <400> 41

<210> 42 <210> 42

<211> 9 <211> 9

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 42 <400> 42

<210> 43 <210> 43

<211> 9 <211> 9

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 43 <400> 43

<210> 44 <210> 44

<211> 8 <211> 8

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 44 <400> 44

<210> 45 <210> 45

<211> 8 <211> 8

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 45 <400> 45

<210> 46 <210> 46

<211> 8 <211> 8

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 46 <400> 46

<210> 47 <210> 47

<211> 9 <211> 9

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 47 <400> 47

<210> 48 <210> 48

<211> 10 <211> 10

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 48 <400> 48

<210> 49 <210> 49

<211> 10 <211> 10

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 49 <400> 49

<210> 50 <210> 50

<211> 10 <211> 10

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 50 <400> 50

<210> 51 <210> 51

<211> 10 <211> 10

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 51 <400> 51

<210> 52 <210> 52

<211> 10 <211> 10

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 52 <400> 52

<210> 53 <210> 53

<211> 10 <211> 10

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 53 <400> 53

<210> 54 <210> 54

<211> 10 <211> 10

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 54 <400> 54

<210> 55 <210> 55

<211> 10 <211> 10

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 55 <400> 55

<210> 56 <210> 56

<211> 10 <211> 10

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 56 <400> 56

<210> 57 <210> 57

<211> 19 <211> 19

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 57 <400> 57

<210> 58 <210> 58

<211> 19 <211> 19

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 58 <400> 58

<210> 59 <210> 59

<211> 19 <211> 19

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 59 <400> 59

<210> 60 <210> 60

<211> 19 <211> 19

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 60 <400> 60

<210> 61 <210> 61

<211> 19 <211> 19

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 61 <400> 61

<210> 62 <210> 62

<211> 19 <211> 19

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 62 <400> 62

<210> 63 <210> 63

<211> 19 <211> 19

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 63 <400> 63

<210> 64 <210> 64

<211> 19 <211> 19

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 64 <400> 64

<210> 65 <210> 65

<211> 19 <211> 19

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 65 <400> 65

<210> 66 <210> 66

<211> 19 <211> 19

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 66 <400> 66

<210> 67 <210> 67

<211> 12 <211> 12

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 67 <400> 67

<210> 68 <210> 68

<211> 5 <211> 5

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 68 <400> 68

<210> 69 <210> 69

<211> 5 <211> 5

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 69 <400> 69

<210> 70 <210> 70

<211> 5 <211> 5

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 70 <400> 70

<210> 71 <210> 71

<211> 5 <211> 5

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 71 <400> 71

<210> 72 <210> 72

<211> 5 <211> 5

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 72 <400> 72

<210> 73 <210> 73

<211> 8 <211> 8

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 73 <400> 73

<210> 74 <210> 74

<211> 8 <211> 8

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 74 <400> 74

<210> 75 <210> 75

<211> 24 <211> 24

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成引子 <223> Description of artificial sequence: synthetic primer

<400> 75 <400> 75

<210> 76 <210> 76

<211> 24 <211> 24

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成引子 <223> Description of artificial sequence: synthetic primer

<400> 76 <400> 76

<210> 77 <210> 77

<211> 21 <211> 21

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成引子 <223> Description of artificial sequence: synthetic primer

<400> 77 <400> 77

<210> 78 <210> 78

<211> 24 <211> 24

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成引子 <223> Description of artificial sequence: synthetic primer

<400> 78 <400> 78

<210> 79 <210> 79

<211> 21 <211> 21

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成引子 <223> Description of artificial sequence: synthetic primer

<400> 79 <400> 79

<210> 80 <210> 80

<211> 24 <211> 24

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成引子 <223> Description of artificial sequence: synthetic primer

<400> 80 <400> 80

<210> 81 <210> 81

<211> 25 <211> 25

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成引子 <223> Description of artificial sequence: synthetic primer

<400> 81 <400> 81

<210> 82 <210> 82

<211> 21 <211> 21

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成引子 <223> Description of artificial sequence: synthetic primer

<400> 82 <400> 82

<210> 83 <210> 83

<211> 24 <211> 24

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成引子 <223> Description of artificial sequence: synthetic primer

<400> 83 <400> 83

<210> 84 <210> 84

<211> 24 <211> 24

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成引子 <223> Description of artificial sequence: synthetic primer

<400> 84 <400> 84

<210> 85 <210> 85

<211> 30 <211> 30

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成引子 <223> Description of artificial sequence: synthetic primer

<400> 85 <400> 85

<210> 86 <210> 86

<211> 20 <211> 20

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成引子 <223> Description of artificial sequence: synthetic primer

<220> <220>

<221> 修飾鹼基 <221> modified base

<222> (6)..(6) <222> (6)..(6)

<223> a,c,t,g,未知或其他 <223> a, c, t, g, unknown or other

<400> 86 <400> 86

<210> 87 <210> 87

<211> 23 <211> 23

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成引子 <223> Description of artificial sequence: synthetic primer

<220> <220>

<221> 修飾鹼基 <221> modified base

<222> (6)..(6) <222> (6)..(6)

<223> a,c,t,g,未知或其他 <223> a, c, t, g, unknown or other

<400> 87 <400> 87

<210> 88 <210> 88

<211> 22 <211> 22

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成引子 <223> Description of artificial sequence: synthetic primer

<400> 88 <400> 88

<210> 89 <210> 89

<211> 20 <211> 20

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成引子 <223> Description of artificial sequence: synthetic primer

<400> 89 <400> 89

<210> 90 <210> 90

<211> 20 <211> 20

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成引子 <223> Description of artificial sequence: synthetic primer

<400> 90 <400> 90

<210> 91 <210> 91

<211> 20 <211> 20

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成引子 <223> Description of artificial sequence: synthetic primer

<400> 91 <400> 91

<210> 92 <210> 92

<211> 20 <211> 20

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成引子 <223> Description of artificial sequence: synthetic primer

<400> 92 <400> 92

<210> 93 <210> 93

<211> 27 <211> 27

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成引子 <223> Description of artificial sequence: synthetic primer

<400> 93 <400> 93

<210> 94 <210> 94

<211> 23 <211> 23

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成引子 <223> Description of artificial sequence: synthetic primer

<400> 94 <400> 94

<210> 95 <210> 95

<211> 24 <211> 24

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成引子 <223> Description of artificial sequence: synthetic primer

<400> 95 <400> 95

<210> 96 <210> 96

<211> 100 <211> 100

<212> PRT <212> PRT

<213> 小鼠類 <213> Mouse

<400> 96 <400> 96

<210> 97 <210> 97

<211> 100 <211> 100

<212> PRT <212> PRT

<213> 智人 <213> Homo sapiens

<400> 97 <400> 97

<210> 98 <210> 98

<211> 100 <211> 100

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 98 <400> 98

<210> 99 <210> 99

<211> 100 <211> 100

<212> PRT <212> PRT

<213> 小鼠類 <213> Mouse

<400> 99 <400> 99

<210> 100 <210> 100

<211> 100 <211> 100

<212> PRT <212> PRT

<213> 智人 <213> Homo sapiens

<400> 100 <400> 100

<210> 101 <210> 101

<211> 100 <211> 100

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 101 <400> 101

<210> 102 <210> 102

<211> 113 <211> 113

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 102 <400> 102

<210> 103 <210> 103

<211> 117 <211> 117

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 103 <400> 103

<210> 104 <210> 104

<211> 12 <211> 12

<212> PRT <212> PRT

<213> 智人 <213> Homo sapiens

<400> 104 <400> 104

<210> 105 <210> 105

<211> 12 <211> 12

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 105 <400> 105

<210> 106 <210> 106

<211> 12 <211> 12

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 106 <400> 106

<210> 107 <210> 107

<211> 12 <211> 12

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 107 <400> 107

<210> 108 <210> 108

<211> 12 <211> 12

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 108 <400> 108

<210> 109 <210> 109

<211> 12 <211> 12

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 109 <400> 109

<210> 110 <210> 110

<211> 12 <211> 12

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 110 <400> 110

<210> 111 <210> 111

<211> 12 <211> 12

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 111 <400> 111

<210> 112 <210> 112

<211> 12 <211> 12

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 112 <400> 112

<210> 113 <210> 113

<211> 12 <211> 12

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 113 <400> 113

<210> 114 <210> 114

<211> 12 <211> 12

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 114 <400> 114

<210> 115 <210> 115

<211> 16 <211> 16

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (1)..(1) <222> (1)..(1)

<223> Lys or Arg <223> Lys or Arg

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (7)..(7) <222> (7)..(7)

<223> Leu,Val or Ile <223> Leu, Val or Ile

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (8)..(8) <222> (8)..(8)

<223> 任何胺基酸 <223> Any amino acid

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (9)..(9) <222> (9)..(9)

<223> Ser or Thr <223> Ser or Thr

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (10)..(10) <222> (10)..(10)

<223> Asn or Asp <223> Asn or Asp

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (12)..(12) <222> (12)..(12)

<223> 任何胺基酸 <223> Any amino acid

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (13)..(13) <222> (13)..(13)

<223> Ser or Thr <223> Ser or Thr

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (16)..(16) <222> (16)..(16)

<223> 任何胺基酸 <223> Any amino acid

<400> 115 <400> 115

<210> 116 <210> 116

<211> 16 <211> 16

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (1)..(1) <222> (1)..(1)

<223> Lys or Arg <223> Lys or Arg

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (7)..(7) <222> (7)..(7)

<223> Leu,Val or Ile <223> Leu, Val or Ile

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (9)..(9) <222> (9)..(9)

<223> Ser or Thr <223> Ser or Thr

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (12)..(12) <222> (12)..(12)

<223> 任何胺基酸 <223> Any amino acid

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (13)..(13) <222> (13)..(13)

<223> Ser or Thr <223> Ser or Thr

<400> 116 <400> 116

<210> 117 <210> 117

<211> 16 <211> 16

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (13)..(13) <222> (13)..(13)

<223> Ser or Thr <223> Ser or Thr

<400> 117 <400> 117

<210> 118 <210> 118

<211> 7 <211> 7

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (1)..(1) <222> (1)..(1)

<223> 任何胺基酸 <223> Any amino acid

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (4)..(6) <222> (4)..(6)

<223> 任何胺基酸 <223> Any amino acid

<400> 118 <400> 118

<210> 119 <210> 119

<211> 7 <211> 7

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (1)..(1) <222> (1)..(1)

<223> 任何胺基酸 <223> Any amino acid

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (4)..(4) <222> (4)..(4)

<223> 任何胺基酸 <223> Any amino acid

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (6)..(6) <222> (6)..(6)

<223> 任何胺基酸 <223> Any amino acid

<400> 119 <400> 119

<210> 120 <210> 120

<211> 7 <211> 7

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (4)..(4) <222> (4)..(4)

<223> 任何胺基酸 <223> Any amino acid

<400> 120 <400> 120

<210> 121 <210> 121

<211> 8 <211> 8

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (1)..(1) <222> (1)..(1)

<223> 任何胺基酸 <223> Any amino acid

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (3)..(3) <222> (3)..(3)

<223> 任何胺基酸 <223> Any amino acid

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (4)..(4) <222> (4)..(4)

<223> 任何胺基酸 <223> Any amino acid

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (5)..(5) <222> (5)..(5)

<223> His,Arg or Lys <223> His, Arg or Lys

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (6)..(6) <222> (6)..(6)

<223> Phe,Leu,Val or Ile <223> Phe, Leu, Val or Ile

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (7)..(8) <222> (7)..(8)

<223> 任何胺基酸 <223> Any amino acid

<400> 121 <400> 121

<210> 122 <210> 122

<211> 8 <211> 8

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (4)..(4) <222> (4)..(4)

<223> 任何胺基酸 <223> Any amino acid

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (5)..(5) <222> (5)..(5)

<223> His,Arg or Lys <223> His, Arg or Lys

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (6)..(6) <222> (6)..(6)

<223> Phe,Leu,Val or Ile <223> Phe, Leu, Val or Ile

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (8)..(8) <222> (8)..(8)

<223> 任何胺基酸 <223> Any amino acid

<400> 122 <400> 122

<210> 123 <210> 123

<211> 8 <211> 8

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (4)..(4) <222> (4)..(4)

<223> 任何胺基酸 <223> Any amino acid

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (8)..(8) <222> (8)..(8)

<223> Phe or Pro <223> Phe or Pro

<400> 123 <400> 123

<210> 124 <210> 124

<211> 10 <211> 10

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (3)..(3) <222> (3)..(3)

<223> 任何胺基酸 <223> Any amino acid

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (5)..(6) <222> (5)..(6)

<223> 任何胺基酸 <223> Any amino acid

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (8)..(8) <222> (8)..(8)

<223> Trp or Tyr <223> Trp or Tyr

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (10)..(10) <222> (10)..(10)

<223> 任何胺基酸 <223> Any amino acid

<400> 124 <400> 124

<210> 125 <210> 125

<211> 10 <211> 10

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (5)..(6) <222> (5)..(6)

<223> 任何胺基酸 <223> Any amino acid

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (8)..(8) <222> (8)..(8)

<223> Trp or Tyr <223> Trp or Tyr

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (10)..(10) <222> (10)..(10)

<223> 任何胺基酸 <223> Any amino acid

<400> 125 <400> 125

<210> 126 <210> 126

<211> 10 <211> 10

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (8)..(8) <222> (8)..(8)

<223> Trp or Tyr <223> Trp or Tyr

<400> 126 <400> 126

<210> 127 <210> 127

<211> 19 <211> 19

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (1)..(1) <222> (1)..(1)

<223> 任何胺基酸 <223> Any amino acid

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (4)..(4) <222> (4)..(4)

<223> 任何胺基酸 <223> Any amino acid

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (6)..(6) <222> (6)..(6)

<223> 任何胺基酸 <223> Any amino acid

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (8)..(8) <222> (8)..(8)

<223> 任何胺基酸 <223> Any amino acid

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (10)..(10) <222> (10)..(10)

<223> 任何胺基酸 <223> Any amino acid

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (12)..(12) <222> (12)..(12)

<223> 任何胺基酸 <223> Any amino acid

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (14)..(15) <222> (14)..(15)

<223> 任何胺基酸 <223> Any amino acid

<400> 127 <400> 127

<210> 128 <210> 128

<211> 19 <211> 19

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (1)..(1) <222> (1)..(1)

<223> 任何胺基酸 <223> Any amino acid

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (4)..(4) <222> (4)..(4)

<223> 任何胺基酸 <223> Any amino acid

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (6)..(6) <222> (6)..(6)

<223> 任何胺基酸 <223> Any amino acid

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (8)..(8) <222> (8)..(8)

<223> 任何胺基酸 <223> Any amino acid

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (14)..(15) <222> (14)..(15)

<223> 任何胺基酸 <223> Any amino acid

<400> 128 <400> 128

<210> 129 <210> 129

<211> 19 <211> 19

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (14)..(15) <222> (14)..(15)

<223> 任何胺基酸 <223> Any amino acid

<400> 129 <400> 129

<210> 130 <210> 130

<211> 5 <211> 5

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (2)..(4) <222> (2)..(4)

<223> 任何胺基酸 <223> Any amino acid

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (5)..(5) <222> (5)..(5)

<223> Tyr,Phe or Trp <223> Tyr, Phe or Trp

<400> 130 <400> 130

<210> 131 <210> 131

<211> 8 <211> 8

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (4)..(4) <222> (4)..(4)

<223> 任何胺基酸 <223> Any amino acid

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (5)..(5) <222> (5)..(5)

<223> Tyr,Phe or Trp <223> Tyr, Phe or Trp

<400> 131 <400> 131

<210> 132 <210> 132

<211> 8 <211> 8

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<220> <220>

<221> MOD_RES <221> MOD_RES

<222> (5)..(5) <222> (5)..(5)

<223> Phe or Trp <223> Phe or Trp

<400> 132 <400> 132

<210> 133 <210> 133

<211> 11 <211> 11

<212> PRT <212> PRT

<213> 智人 <213> Homo sapiens

<400> 133 <400> 133

<210> 134 <210> 134

<211> 10 <211> 10

<212> PRT <212> PRT

<213> 智人 <213> Homo sapiens

<400> 134 <400> 134

<210> 135 <210> 135

<211> 10 <211> 10

<212> PRT <212> PRT

<213> 智人 <213> Homo sapiens

<400> 135 <400> 135

<210> 136 <210> 136

<211> 117 <211> 117

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 136 <400> 136

<210> 137 <210> 137

<211> 117 <211> 117

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 137 <400> 137

<210> 138 <210> 138

<211> 112 <211> 112

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 138 <400> 138

<210> 139 <210> 139

<211> 114 <211> 114

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 139 <400> 139

<210> 140 <210> 140

<211> 114 <211> 114

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 140 <400> 140

<210> 141 <210> 141

<211> 114 <211> 114

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 141 <400> 141

<210> 142 <210> 142

<211> 114 <211> 114

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 142 <400> 142

<210> 143 <210> 143

<211> 114 <211> 114

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 143 <400> 143

<210> 144 <210> 144

<211> 114 <211> 114

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 144 <400> 144

<210> 145 <210> 145

<211> 111 <211> 111

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 145 <400> 145

<210> 146 <210> 146

<211> 111 <211> 111

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 146 <400> 146

<210> 147 <210> 147

<211> 111 <211> 111

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 147 <400> 147

<210> 148 <210> 148

<211> 111 <211> 111

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 148 <400> 148

<210> 149 <210> 149

<211> 114 <211> 114

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 149 <400> 149

<210> 150 <210> 150

<211> 114 <211> 114

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 150 <400> 150

<210> 151 <210> 151

<211> 114 <211> 114

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 151 <400> 151

<210> 152 <210> 152

<211> 114 <211> 114

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 152 <400> 152

<210> 153 <210> 153

<211> 111 <211> 111

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 153 <400> 153

<210> 154 <210> 154

<211> 111 <211> 111

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 154 <400> 154

<210> 155 <210> 155

<211> 111 <211> 111

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 155 <400> 155

<210> 156 <210> 156

<211> 111 <211> 111

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 156 <400> 156

<210> 157 <210> 157

<211> 111 <211> 111

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 157 <400> 157

<210> 158 <210> 158

<211> 113 <211> 113

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 158 <400> 158

<210> 159 <210> 159

<211> 114 <211> 114

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 159 <400> 159

<210> 160 <210> 160

<211> 114 <211> 114

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 160 <400> 160

<210> 161 <210> 161

<211> 114 <211> 114

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 161 <400> 161

<210> 162 <210> 162

<211> 114 <211> 114

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 162 <400> 162

<210> 163 <210> 163

<211> 114 <211> 114

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 163 <400> 163

<210> 164 <210> 164

<211> 112 <211> 112

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 164 <400> 164

<210> 165 <210> 165

<211> 112 <211> 112

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 165 <400> 165

<210> 166 <210> 166

<211> 112 <211> 112

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 166 <400> 166

<210> 167 <210> 167

<211> 112 <211> 112

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 167 <400> 167

<210> 168 <210> 168

<211> 112 <211> 112

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 168 <400> 168

<210> 169 <210> 169

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 169 <400> 169

<210> 170 <210> 170

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 170 <400> 170

<210> 171 <210> 171

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 171 <400> 171

<210> 172 <210> 172

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 172 <400> 172

<210> 173 <210> 173

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 173 <400> 173

<210> 174 <210> 174

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 174 <400> 174

<210> 175 <210> 175

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 175 <400> 175

<210> 176 <210> 176

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 176 <400> 176

<210> 177 <210> 177

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 177 <400> 177

<210> 178 <210> 178

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 178 <400> 178

<210> 179 <210> 179

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 179 <400> 179

<210> 180 <210> 180

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 180 <400> 180

<210> 181 <210> 181

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 智人 <213> Homo sapiens

<400> 181 <400> 181

<210> 182 <210> 182

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 智人 <213> Homo sapiens

<400> 182 <400> 182

<210> 183 <210> 183

<211> 19 <211> 19

<212> PRT <212> PRT

<213> 未知 <213> Unknown

<220> <220>

<223> 未知之描述:破傷風類毒素胜肽 <223> Description of the unknown: tetanus toxoid peptide

<400> 183 <400> 183

<210> 184 <210> 184

<211> 21 <211> 21

<212> PRT <212> PRT

<213> 未知 <213> Unknown

<220> <220>

<223> 未知之描述:破傷風類毒素胜肽 <223> Description of the unknown: tetanus toxoid peptide

<400> 184 <400> 184

<210> 185 <210> 185

<211> 20 <211> 20

<212> PRT <212> PRT

<213> 未知 <213> Unknown

<220> <220>

<223> 未知之描述:破傷風類毒素胜肽 <223> Description of the unknown: tetanus toxoid peptide

<400> 185 <400> 185

<210> 186 <210> 186

<211> 21 <211> 21

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 186 <400> 186

<210> 187 <210> 187

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 187 <400> 187

<210> 188 <210> 188

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 188 <400> 188

<210> 189 <210> 189

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 189 <400> 189

<210> 190 <210> 190

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 190 <400> 190

<210> 191 <210> 191

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 191 <400> 191

<210> 192 <210> 192

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 192 <400> 192

<210> 193 <210> 193

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 193 <400> 193

<210> 194 <210> 194

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 194 <400> 194

<210> 195 <210> 195

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 195 <400> 195

<210> 196 <210> 196

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 196 <400> 196

<210> 197 <210> 197

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 197 <400> 197

<210> 198 <210> 198

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 198 <400> 198

<210> 199 <210> 199

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 199 <400> 199

<210> 200 <210> 200

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 200 <400> 200

<210> 201 <210> 201

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 201 <400> 201

<210> 202 <210> 202

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 202 <400> 202

<210> 203 <210> 203

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 203 <400> 203

<210> 204 <210> 204

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 204 <400> 204

<210> 205 <210> 205

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 205 <400> 205

<210> 206 <210> 206

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 206 <400> 206

<210> 207 <210> 207

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 207 <400> 207

<210> 208 <210> 208

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 208 <400> 208

<210> 209 <210> 209

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 209 <400> 209

<210> 210 <210> 210

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 210 <400> 210

<210> 211 <210> 211

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 211 <400> 211

<210> 212 <210> 212

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 212 <400> 212

<210> 213 <210> 213

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 213 <400> 213

<210> 214 <210> 214

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 214 <400> 214

<210> 215 <210> 215

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 215 <400> 215

<210> 216 <210> 216

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 216 <400> 216

<210> 217 <210> 217

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 217 <400> 217

<210> 218 <210> 218

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 218 <400> 218

<210> 219 <210> 219

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 219 <400> 219

<210> 220 <210> 220

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 220 <400> 220

<210> 221 <210> 221

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 221 <400> 221

<210> 222 <210> 222

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 222 <400> 222

<210> 223 <210> 223

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 223 <400> 223

<210> 224 <210> 224

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 224 <400> 224

<210> 225 <210> 225

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 225 <400> 225

<210> 226 <210> 226

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 226 <400> 226

<210> 227 <210> 227

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 227 <400> 227

<210> 228 <210> 228

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 228 <400> 228

<210> 229 <210> 229

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 229 <400> 229

<210> 230 <210> 230

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 230 <400> 230

<210> 231 <210> 231

<211> 14 <211> 14

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 231 <400> 231

<210> 232 <210> 232

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 232 <400> 232

<210> 233 <210> 233

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 233 <400> 233

<210> 234 <210> 234

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 234 <400> 234

<210> 235 <210> 235

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 235 <400> 235

<210> 236 <210> 236

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 236 <400> 236

<210> 237 <210> 237

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 237 <400> 237

<210> 238 <210> 238

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 238 <400> 238

<210> 239 <210> 239

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 239 <400> 239

<210> 240 <210> 240

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 240 <400> 240

<210> 241 <210> 241

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 241 <400> 241

<210> 242 <210> 242

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 242 <400> 242

<210> 243 <210> 243

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 243 <400> 243

<210> 244 <210> 244

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 244 <400> 244

<210> 245 <210> 245

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 245 <400> 245

<210> 246 <210> 246

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 246 <400> 246

<210> 247 <210> 247

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 247 <400> 247

<210> 248 <210> 248

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 248 <400> 248

<210> 249 <210> 249

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 249 <400> 249

<210> 250 <210> 250

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 250 <400> 250

<210> 251 <210> 251

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 251 <400> 251

<210> 252 <210> 252

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 252 <400> 252

<210> 253 <210> 253

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 253 <400> 253

<210> 254 <210> 254

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 254 <400> 254

<210> 255 <210> 255

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 255 <400> 255

<210> 256 <210> 256

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 256 <400> 256

<210> 257 <210> 257

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 257 <400> 257

<210> 258 <210> 258

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 258 <400> 258

<210> 259 <210> 259

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 259 <400> 259

<210> 260 <210> 260

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 260 <400> 260

<210> 261 <210> 261

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 261 <400> 261

<210> 262 <210> 262

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 262 <400> 262

<210> 263 <210> 263

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 263 <400> 263

<210> 264 <210> 264

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 264 <400> 264

<210> 265 <210> 265

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 265 <400> 265

<210> 266 <210> 266

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 266 <400> 266

<210> 267 <210> 267

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 267 <400> 267

<210> 268 <210> 268

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 268 <400> 268

<210> 269 <210> 269

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 269 <400> 269

<210> 270 <210> 270

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 270 <400> 270

<210> 271 <210> 271

<211> 15 <211> 15

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 271 <400> 271

<210> 272 <210> 272

<211> 464 <211> 464

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 272 <400> 272

<210> 273 <210> 273

<211> 238 <211> 238

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 273 <400> 273

<210> 274 <210> 274

<211> 467 <211> 467

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 274 <400> 274

<210> 275 <210> 275

<211> 239 <211> 239

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 275 <400> 275

<210> 276 <210> 276

<211> 464 <211> 464

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 276 <400> 276

<210> 277 <210> 277

<211> 464 <211> 464

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 277 <400> 277

<210> 278 <210> 278

<211> 239 <211> 239

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 278 <400> 278

<210> 279 <210> 279

<211> 464 <211> 464

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 279 <400> 279

<210> 280 <210> 280

<211> 238 <211> 238

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 280 <400> 280

<210> 281 <210> 281

<211> 467 <211> 467

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 281 <400> 281

<210> 282 <210> 282

<211> 240 <211> 240

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成多肽 <223> Description of the artificial sequence: synthetic peptide

<400> 282 <400> 282

<210> 283 <210> 283

<211> 1395 <211> 1395

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成聚核苷酸 <223> Description of Artificial Sequence: Synthetic Polynucleotide

<400> 283 <400> 283

<210> 284 <210> 284

<211> 717 <211> 717

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成聚核苷酸 <223> Description of Artificial Sequence: Synthetic Polynucleotide

<400> 284 <400> 284

<210> 285 <210> 285

<211> 1404 <211> 1404

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成聚核苷酸 <223> Description of Artificial Sequence: Synthetic Polynucleotide

<400> 285 <400> 285

<210> 286 <210> 286

<211> 720 <211> 720

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成聚核苷酸 <223> Description of Artificial Sequence: Synthetic Polynucleotide

<400> 286 <400> 286

<210> 287 <210> 287

<211> 1395 <211> 1395

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成聚核苷酸 <223> Description of Artificial Sequence: Synthetic Polynucleotide

<220> <220>

<221> 修飾鹼基 <221> modified base

<222> (1398)..(1398) <222> (1398)..(1398)

<223> a,c,t,g,未知或其他 <223> a, c, t, g, unknown or other

<400> 287 <400> 287

<210> 288 <210> 288

<211> 1395 <211> 1395

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成聚核苷酸 <223> Description of Artificial Sequence: Synthetic Polynucleotide

<220> <220>

<221> 修飾鹼基 <221> modified base

<222> (1398)..(1398) <222> (1398)..(1398)

<223> a,c,t,g,未知或其他 <223> a, c, t, g, unknown or other

<400> 288 <400> 288

<210> 289 <210> 289

<211> 720 <211> 720

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成聚核苷酸 <223> Description of Artificial Sequence: Synthetic Polynucleotide

<400> 289 <400> 289

<210> 290 <210> 290

<211> 1395 <211> 1395

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成聚核苷酸 <223> Description of Artificial Sequence: Synthetic Polynucleotide

<400> 290 <400> 290

<210> 291 <210> 291

<211> 717 <211> 717

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成聚核苷酸 <223> Description of Artificial Sequence: Synthetic Polynucleotide

<400> 291 <400> 291

<210> 292 <210> 292

<211> 1404 <211> 1404

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成聚核苷酸 <223> Description of Artificial Sequence: Synthetic Polynucleotide

<400> 292 <400> 292

<210> 293 <210> 293

<211> 723 <211> 723

<212> DNA <212> DNA

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成聚核苷酸 <223> Description of Artificial Sequence: Synthetic Polynucleotide

<400> 293 <400> 293

<210> 294 <210> 294

<211> 8 <211> 8

<212> PRT <212> PRT

<213> 人工序列 <213> Artificial sequence

<220> <220>

<223> 人工序列之描述:合成胜肽 <223> Description of artificial sequence: synthetic peptide

<400> 294 <400> 294

(無元件符號說明)(no component symbol description)

Claims (36)

一種單株抗-人類CD52抗體或結合人類CD52的抗原-結合部份,其中該抗體之重鏈(H)-CDR1、H-CDR2、H-CDR3及輕鏈(L)-CDR1、L-CDR2、及L-CDR3分別包含SEQ ID NOs:53、63、71、31、36及44之胺基酸序列。 A monoclonal anti-human CD52 antibody or an antigen-binding portion of human CD52, wherein the heavy chain (H)-CDR1, H-CDR2, H-CDR3 and light chain (L)-CDR1, L-CDR2 of the antibody And L-CDR3 comprise the amino acid sequences of SEQ ID NOs: 53, 63, 71, 31, 36 and 44, respectively. 一種單株抗-人類CD52抗體或結合人類CD52的抗原-結合部份,其中該抗體的重鏈及輕鏈分別包含SEQ ID NOs:279及280的胺基酸序列,且無信號序列。 A monoclonal anti-human CD52 antibody or an antigen-binding portion that binds to human CD52, wherein the heavy and light chains of the antibody comprise the amino acid sequences of SEQ ID NOs: 279 and 280, respectively, and have no signal sequence. 如請求項1之單株抗-人類CD52抗體或抗原-結合部份,其中該抗體的輕鏈包含自SEQ ID NOs:153-157所組成的群組中選出的胺基酸序列。 The monoclonal anti-human CD52 antibody or antigen-binding portion of claim 1, wherein the light chain of the antibody comprises an amino acid sequence selected from the group consisting of SEQ ID NOs: 153-157. 如請求項1之單株抗-人類CD52抗體或抗原-結合部份,其中該抗體的輕鏈包含SEQ ID NO:280的胺基酸序列,且無信號序列。 The monoclonal anti-human CD52 antibody or antigen-binding portion of claim 1, wherein the light chain of the antibody comprises the amino acid sequence of SEQ ID NO: 280 and has no signal sequence. 如請求項1之單株抗-人類CD52抗體或抗原-結合部分,其中該抗體的重鏈包含自SEQ ID NOs:149-152所組成的群組中選出的胺基酸序列。 The monoclonal anti-human CD52 antibody or antigen-binding portion of claim 1, wherein the heavy chain of the antibody comprises an amino acid sequence selected from the group consisting of SEQ ID NOs: 149-152. 如請求項1之單株抗-人類CD52抗體或抗原-結合部份,其中該抗體的重鏈包含SEQ ID NO:279的胺基酸序列,且無信號序列。 The monoclonal anti-human CD52 antibody or antigen-binding portion of claim 1, wherein the heavy chain of the antibody comprises the amino acid sequence of SEQ ID NO: 279 and has no signal sequence. 如請求項1-6中任一項之單株抗-人類CD52抗體或抗原-結合部份,其中該抗體係為人類化抗體、老鼠抗體或嵌合抗體。 The monoclonal anti-human CD52 antibody or antigen-binding portion of any one of claims 1 to 6, wherein the anti-system is a humanized antibody, a mouse antibody or a chimeric antibody. 如請求項1-6中任一項之單株抗-人類CD52抗體或抗原-結 合部份,其中該重鏈的骨架區使用VH3-72或VH3-23人類生殖株序列,且其中該輕鏈的骨架區使用VK2 A18b人類生殖株序列。 A monoclonal anti-human CD52 antibody or antigen-knot according to any one of claims 1-6 In part, wherein the framework region of the heavy chain uses the VH3-72 or VH3-23 human reproductive strain sequence, and wherein the framework region of the light chain uses the VK2 A18b human reproductive strain sequence. 如請求項1-6中任一項之單株抗-人類CD52抗體或抗原-結合部份,其中該抗體的輕鏈及重鏈分別包含SEQ ID NOs:9及22之胺基酸序列。 The monoclonal anti-human CD52 antibody or antigen-binding portion of any one of claims 1 to 6, wherein the light and heavy chains of the antibody comprise the amino acid sequences of SEQ ID NOs: 9 and 22, respectively. 如請求項1-6中任一項之單株抗-人類CD52抗體或抗原-結合部份,其中該重鏈及輕鏈包含胺基酸序列a)分別為SEQ ID NOs:149及155;或b)分別為SEQ ID NOs:149及156。 The monoclonal anti-human CD52 antibody or antigen-binding portion of any one of claims 1 to 6, wherein the heavy chain and the light chain comprise an amino acid sequence a) are SEQ ID NOs: 149 and 155, respectively; b) are SEQ ID NOs: 149 and 156, respectively. 如請求項1、3及5中任一項的單株抗-人類CD52抗體或抗原-結合部份,其中該抗體為IgG1、IgG2、IgG3或IgG4分子。 The monoclonal anti-human CD52 antibody or antigen-binding portion of any one of claims 1, 3 and 5, wherein the antibody is an IgG1, IgG2, IgG3 or IgG4 molecule. 如請求項1、3及5中任一項的單株抗-人類CD52抗體或抗原-結合部份,其中該部份係為單鏈抗體、Fv、Fab、Fab'、F(ab')2、Fd、單鏈Fv分子(scFv)、雙特定單鏈Fv二聚體、雙鏈抗體、區域缺失抗體或單域抗體(dAb)。 The monoclonal anti-human CD52 antibody or antigen-binding portion according to any one of claims 1, 3 and 5, wherein the portion is a single chain antibody, Fv, Fab, Fab', F(ab') 2 , Fd, single chain Fv molecule (scFv), bispecific single chain Fv dimer, double chain antibody, region deleted antibody or single domain antibody (dAb). 如請求項1-6中任一項之單株抗-人類CD52抗體或抗原-結合部份,其中所述抗體或部份係結合至包含SEQ ID NO:104的胺基酸序列,且視情況,該抗體或部分至SEQ ID NO:104的結合係由在SEQ ID NO:104的殘基殘基4、7、8或11的丙胺酸取代所還原。 The monoclonal anti-human CD52 antibody or antigen-binding portion of any one of claims 1 to 6, wherein the antibody or portion binds to an amino acid sequence comprising SEQ ID NO: 104, and optionally The antibody or a portion of the binding line to SEQ ID NO: 104 is reduced by alanine substitution at residue 4, 7, 8, or 11 of SEQ ID NO: 104. 如請求項1-6中任一項的單株抗-人類CD52抗體或抗原-結合部份,其中該抗體或抗原-結合部份具有自下列所組成 的群組中選出的一或更多性質:a)消耗T或B淋巴細胞,或二者;b)與B淋巴細胞相較,優先地消耗T淋巴細胞;c)增加TNF-α、IL-6、或MCP-1的循環血清含量;d)介導CD52-表現細胞的抗體-依賴細胞介導性細胞毒性(ADCC);e)介導CD52-表現細胞的補體依賴細胞毒性(CDC);f)於阿來組單抗(alemtuzumab)中和抗體存在下結合人類CD52;及g)促進人類T及/或B細胞的細胞內發信號,或二者。 The monoclonal anti-human CD52 antibody or antigen-binding portion according to any one of claims 1 to 6, wherein the antibody or antigen-binding portion has the following composition One or more properties selected from the group: a) consumption of T or B lymphocytes, or both; b) preferential consumption of T lymphocytes compared to B lymphocytes; c) increase of TNF-α, IL- 6. Circulating serum content of MCP-1; d) antibody-dependent cell-mediated cytotoxicity (ADCC) mediated by CD52-expressing cells; e) mediating complement-dependent cytotoxicity (CDC) of CD52-expressing cells; f) binding to human CD52 in the presence of an alemtuzumab neutralizing antibody; and g) promoting intracellular signaling of human T and/or B cells, or both. 一種組合物,其包含如請求項1-14中任一項的單株抗-人類CD52抗體或抗原-結合部分,以及醫藥上可接受媒劑或載劑。 A composition comprising a monoclonal anti-human CD52 antibody or antigen-binding portion according to any one of claims 1-14, and a pharmaceutically acceptable vehicle or carrier. 一種經分離核酸,其編碼如請求項1-14中任一項的單株抗-人類CD52抗體或抗原-結合部分的重鏈或輕鏈或兩者。 An isolated nucleic acid encoding the heavy or light chain or both of the monoclonal anti-human CD52 antibody or antigen-binding portion of any of claims 1-14. 如請求項16的經分離核酸,其中該經分離核酸係包含:a)SEQ ID NO:290的重鏈核苷酸序列,或是該核苷酸序列不具編碼信號胜肽的序列;b)SEQ ID NO:291的輕鏈核苷酸序列,或是該核苷酸序列不具編碼信號胜肽的序列;或是c)a)及b)兩者的核苷酸序列。 The isolated nucleic acid of claim 16, wherein the isolated nucleic acid vector comprises: a) a heavy chain nucleotide sequence of SEQ ID NO: 290, or a sequence in which the nucleotide sequence does not encode a signal peptide; b) SEQ ID NO: The light chain nucleotide sequence of 291, or the sequence in which the nucleotide sequence does not have a signal peptide; or the nucleotide sequence of c) a) and b). 如請求項17的經分離核酸,其中該經分離核酸包含分別為SEQ ID NO:290及SEQ ID NO:291的重鏈核苷酸序列 與輕鏈核苷酸序列,兩者皆不具編碼信號胜肽的序列。 The isolated nucleic acid of claim 17, wherein the isolated nucleic acid comprises a heavy chain nucleotide sequence of SEQ ID NO: 290 and SEQ ID NO: 291, respectively And the light chain nucleotide sequence, neither of which has a sequence encoding a signal peptide. 一種宿主細胞,其包含編碼如請求項1-14中任一項的單株抗-人類CD52抗體或抗原-結合部分的重鏈的第一核酸序列,該第一核酸序列係操作地鏈結至表現控制因子,以及編碼所述單株抗體或抗原-結合部分的輕鏈的第二核酸序列,該第二核酸序列係操作地鏈結至表現控制因子。 A host cell comprising a first nucleic acid sequence encoding a heavy chain of a monoclonal anti-human CD52 antibody or antigen-binding portion of any one of claims 1-14, operatively linked to A performance control factor, and a second nucleic acid sequence encoding the light chain of the monoclonal antibody or antigen-binding portion of the monoclonal antibody, the second nucleic acid sequence being operatively linked to a performance control factor. 一種表現抗-人類CD52抗體或結合人類CD52的抗原-結合部分的方法,其包含在適合所述抗體或部分表現的條件下培養請求項19的該宿主細胞,及表現該抗體或部分。 A method of expressing an anti-human CD52 antibody or binding to an antigen-binding portion of human CD52, comprising culturing the host cell of claim 19 under conditions suitable for the expression of the antibody or part, and expressing the antibody or portion. 一種如請求項1-14中任一項的單株抗-人類CD52抗體或抗原-結合部分之用途,其係用於製備在需要的病人中誘發免疫抑制的藥物。 Use of a monoclonal anti-human CD52 antibody or antigen-binding portion according to any one of claims 1-14 for the preparation of a medicament for inducing immunosuppression in a patient in need thereof. 如請求項21之用途,其中該病人係具自體免疫疾病。 The use of claim 21, wherein the patient has an autoimmune disease. 一種如請求項1-14中任一項的單株抗-人類CD52抗體或抗原-結合部分之用途,其係用於製備在癌症病人中靶向CD52+細胞的藥物。 Use of a monoclonal anti-human CD52 antibody or antigen-binding portion according to any one of claims 1-14 for the preparation of a medicament for targeting CD52 + cells in a cancer patient. 一種如請求項1-14中任一項的單株抗-人類CD52抗體或抗原-結合部分之用途,其係用於製備在需要的病人中抑制血管生成的藥物。 Use of a monoclonal anti-human CD52 antibody or antigen-binding portion according to any one of claims 1-14 for the preparation of a medicament for inhibiting angiogenesis in a patient in need thereof. 如請求項21的用途,其中該病人係接受移植。 The use of claim 21, wherein the patient is transplanted. 如請求項22之用途,其中該自體免疫疾病係為多發性硬化症、風濕性關節炎、系統性紅斑狼瘡或血管炎。 The use of claim 22, wherein the autoimmune disease is multiple sclerosis, rheumatoid arthritis, systemic lupus erythematosus or vasculitis. 如請求項23之用途,其中該癌症病人係具白血病。 The use of claim 23, wherein the cancer patient has leukemia. 如請求項23之用途,其中該癌症病人係具淋巴瘤。 The use of claim 23, wherein the cancer patient has a lymphoma. 如請求項23之用途,其中該癌症病人係具T細胞惡性腫瘤,且與B細胞相較,該抗體或部分優先地消耗T細胞。 The use of claim 23, wherein the cancer patient has a T cell malignancy and the antibody or portion preferentially consumes T cells as compared to the B cell. 如請求項23之用途,其中該癌症病人係具實體腫瘤。 The use of claim 23, wherein the cancer patient has a solid tumor. 如請求項21之用途,其中該藥物進一步包含嗜中性球或NK細胞刺激劑。 The use of claim 21, wherein the medicament further comprises a neutrophil or NK cell stimulating agent. 如請求項23之用途,其中該藥物進一步包含嗜中性球或NK細胞刺激劑。 The use of claim 23, wherein the medicament further comprises a neutrophil or NK cell stimulating agent. 如請求項21之用途,其中該藥物進一步包含T調節細胞刺激劑 The use of claim 21, wherein the medicament further comprises a T regulatory cell stimulating agent 如請求項23之用途,其中該藥物進一步包含T調節細胞刺激劑。 The use of claim 23, wherein the medicament further comprises a T regulatory cell stimulating agent. 如請求項24的用途,其中該病人係具實體腫瘤。 The use of claim 24, wherein the patient is a solid tumor. 如請求項24的用途,其中該病人係具血管新生。 The use of claim 24, wherein the patient is angiogenic.
TW099115371A 2009-05-13 2010-05-13 Anti-human cd52 immunoglobulins TWI529247B (en)

Applications Claiming Priority (1)

Application Number Priority Date Filing Date Title
US17783709P 2009-05-13 2009-05-13

Publications (2)

Publication Number Publication Date
TW201043694A TW201043694A (en) 2010-12-16
TWI529247B true TWI529247B (en) 2016-04-11

Family

ID=43085579

Family Applications (3)

Application Number Title Priority Date Filing Date
TW099115371A TWI529247B (en) 2009-05-13 2010-05-13 Anti-human cd52 immunoglobulins
TW104144762A TWI614267B (en) 2009-05-13 2010-05-13 Anti-human cd52 immunoglobulins
TW106123171A TW201825115A (en) 2009-05-13 2010-05-13 Anti-human cd52 immunoglobulins

Family Applications After (2)

Application Number Title Priority Date Filing Date
TW104144762A TWI614267B (en) 2009-05-13 2010-05-13 Anti-human cd52 immunoglobulins
TW106123171A TW201825115A (en) 2009-05-13 2010-05-13 Anti-human cd52 immunoglobulins

Country Status (19)

Country Link
US (5) US8617554B2 (en)
EP (3) EP3683317A3 (en)
JP (4) JP5894912B2 (en)
KR (5) KR101537840B1 (en)
CN (3) CN102459628A (en)
AR (1) AR076770A1 (en)
AU (1) AU2010249003B2 (en)
BR (1) BRPI1013085A2 (en)
CA (2) CA2939492C (en)
HK (2) HK1222682A1 (en)
IL (2) IL216141B (en)
MX (1) MX2011012047A (en)
MY (1) MY160126A (en)
NZ (2) NZ596384A (en)
RU (2) RU2603743C2 (en)
SG (2) SG176060A1 (en)
TW (3) TWI529247B (en)
WO (1) WO2010132659A2 (en)
ZA (1) ZA201108077B (en)

Families Citing this family (34)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
EP2300022A2 (en) 2008-04-25 2011-03-30 Duke University Regulatory b cells and their uses
TWI529247B (en) 2009-05-13 2016-04-11 建新公司 Anti-human cd52 immunoglobulins
EP3345620B1 (en) 2009-05-13 2024-08-28 Genzyme Corporation Methods and compositions for treating lupus
WO2012088272A1 (en) * 2010-12-21 2012-06-28 Duke University Methods and compositions combining immunotherapy with monocyte activation
JP6104794B2 (en) 2011-04-18 2017-03-29 国立大学法人 東京大学 Diagnosis and treatment of cancer using anti-ITM2A antibody
GB201109238D0 (en) 2011-06-01 2011-07-13 Antitope Ltd Antibodies
BR112014009925B1 (en) 2011-10-28 2022-09-20 Teva Pharmaceuticals Australia Pty Ltd POLYPEPTIDE BUILDERS AND THEIR USES
WO2013185165A1 (en) * 2012-06-14 2013-12-19 The Walter And Eliza Hall Institute Of Medical Research Cd-52 antibodies and their use in determining and enhancing an immune response in a subject
US10017739B2 (en) 2012-09-06 2018-07-10 Duke University Methods of expanding and assessing B cells and using expanded B cells to treat disease
US20150299315A1 (en) * 2012-10-22 2015-10-22 Becton, Dickinson And Company Non-b-lineage cells capable of producing antibody
US10365275B2 (en) 2013-03-12 2019-07-30 Institute of Arthritis Reasearch, LLC Immunologically active polypeptide
CA2902026C (en) 2013-03-13 2023-08-29 Prothena Biosciences Limited Tau immunotherapy
AR095199A1 (en) * 2013-03-15 2015-09-30 Genzyme Corp ANTI-CD52 ANTIBODIES
KR102042174B1 (en) 2013-03-29 2019-11-08 삼성전자주식회사 Humanized and affinity-matured anti c-Met antibody and uses thereof
KR102060540B1 (en) * 2013-04-03 2019-12-31 삼성전자주식회사 Pharmaceutical composition for a combination therapy containing an anti-c-Met antibody and anti-Ang2 antibody
JP6433085B2 (en) 2013-04-09 2018-12-05 ボストン バイオメディカル, インコーポレイテッド 2-acetylnaphtho [2,3-b] furan-4,9-dione for use in the treatment of cancer
KR102186363B1 (en) * 2013-09-06 2020-12-04 삼성전자주식회사 Pharmaceutical composition for combination therapy containing c-Met inhibitor and beta-catenin inhibitor
KR102192591B1 (en) * 2013-09-09 2020-12-18 삼성전자주식회사 Pharmaceutical composition for combination therapy containing c-Met inhibitor and c-Myc inhibitor
EA201792623A1 (en) 2015-06-03 2018-04-30 Бостон Биомедикал, Инк. COMPOSITIONS CONTAINING CANCER STEM BONE INHIBITOR AND IMMUNOTHERAPEUTIC AGENT TO BE USED IN CANCER TREATMENT
CN109415432B (en) 2016-05-02 2022-07-08 普罗塞纳生物科学有限公司 TAU immunotherapy
CN109219615B (en) 2016-05-02 2022-12-09 普罗塞纳生物科学有限公司 Antibodies recognizing TAU
SG11201809331RA (en) 2016-05-02 2018-11-29 Prothena Biosciences Ltd Antibodies recognizing tau
JP7106563B2 (en) 2016-11-29 2022-07-26 スミトモ ファーマ オンコロジー, インコーポレイテッド Naphthofuran derivatives, their preparation and methods of use
EP3554515A4 (en) 2016-12-15 2020-08-26 Duke University Antibodies and methods for depleting regulatory b10 cells and use in combination with immune checkpoint inhibitors
US20200299399A1 (en) * 2017-04-21 2020-09-24 Genzyme Corporation Treatment of Multiple Sclerosis with Anti-CD52 Antibodies
BR112019022906A2 (en) 2017-05-02 2020-05-26 Prothena Biosciences Limited ANTIBODIES THAT RECOGNIZE TAU
WO2018213424A1 (en) 2017-05-17 2018-11-22 Boston Biomedical, Inc. Methods for treating cancer
GB201710836D0 (en) * 2017-07-05 2017-08-16 Ucl Business Plc ROR1 Car T-Cells
KR20200103751A (en) * 2017-12-20 2020-09-02 라디뮨 테라퓨틱스 인코포레이티드 Antibodies to Centrin-1, methods for preparing the same, and uses
FI3898668T3 (en) * 2018-12-19 2023-11-28 Humabs Biomed Sa Antibodies that neutralize hepatitis b virus and uses thereof
JP2022524588A (en) 2019-03-03 2022-05-09 プロセナ バイオサイエンシーズ リミテッド Tau recognition antibody
CN109929835A (en) * 2019-03-27 2019-06-25 中国人民解放军第四军医大学 A kind of amplification method of mouse monoclonal antibody function light-chain variable region gene
WO2021223719A1 (en) * 2020-05-08 2021-11-11 亘喜生物科技(上海)有限公司 Antibody directed against cd19 antibody, and preparation therefor and application thereof
AR124414A1 (en) 2020-12-18 2023-03-22 Century Therapeutics Inc CHIMERIC ANTIGEN RECEPTOR SYSTEM WITH ADAPTABLE RECEPTOR SPECIFICITY

Family Cites Families (75)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
GB8308235D0 (en) 1983-03-25 1983-05-05 Celltech Ltd Polypeptides
US4816567A (en) 1983-04-08 1989-03-28 Genentech, Inc. Recombinant immunoglobin preparations
US6054561A (en) * 1984-02-08 2000-04-25 Chiron Corporation Antigen-binding sites of antibody molecules specific for cancer antigens
GB8422238D0 (en) 1984-09-03 1984-10-10 Neuberger M S Chimeric proteins
US4970198A (en) 1985-10-17 1990-11-13 American Cyanamid Company Antitumor antibiotics (LL-E33288 complex)
GB8607679D0 (en) 1986-03-27 1986-04-30 Winter G P Recombinant dna product
US5225539A (en) 1986-03-27 1993-07-06 Medical Research Council Recombinant altered antibodies and methods of making altered antibodies
WO1987006265A1 (en) 1986-04-17 1987-10-22 Kyowa Hakko Kogyo Co., Ltd. Novel compounds dc-88a and dc-89a1 and process for their preparation
US4946778A (en) 1987-09-21 1990-08-07 Genex Corporation Single polypeptide chain binding molecules
WO1988007089A1 (en) 1987-03-18 1988-09-22 Medical Research Council Altered antibodies
AU612370B2 (en) 1987-05-21 1991-07-11 Micromet Ag Targeted multifunctional proteins
WO1989007142A1 (en) 1988-02-05 1989-08-10 Morrison Sherie L Domain-modified constant region antibodies
WO1989007452A1 (en) 1988-02-12 1989-08-24 Medical Research Council Improvements in or relating to antibodies
US5530101A (en) 1988-12-28 1996-06-25 Protein Design Labs, Inc. Humanized immunoglobulins
JP2598116B2 (en) 1988-12-28 1997-04-09 協和醗酵工業株式会社 New substance DC113
JP2510335B2 (en) 1989-07-03 1996-06-26 協和醗酵工業株式会社 DC-88A derivative
US5187186A (en) 1989-07-03 1993-02-16 Kyowa Hakko Kogyo Co., Ltd. Pyrroloindole derivatives
US5208020A (en) 1989-10-25 1993-05-04 Immunogen Inc. Cytotoxic agents comprising maytansinoids and their therapeutic use
DK0814159T3 (en) 1990-08-29 2005-10-24 Genpharm Int Transgenic, non-human animals capable of forming heterologous antibodies
GB9022547D0 (en) 1990-10-17 1990-11-28 Wellcome Found Purified immunoglobulin
GB9022543D0 (en) 1990-10-17 1990-11-28 Wellcome Found Antibody production
GB9108056D0 (en) * 1991-04-16 1991-06-05 Hale Geoffrey Synthetic antigen
DE69233482T2 (en) 1991-05-17 2006-01-12 Merck & Co., Inc. Method for reducing the immunogenicity of antibody variable domains
EP0940468A1 (en) 1991-06-14 1999-09-08 Genentech, Inc. Humanized antibody variable domain
WO1994004679A1 (en) 1991-06-14 1994-03-03 Genentech, Inc. Method for making humanized antibodies
US5264586A (en) 1991-07-17 1993-11-23 The Scripps Research Institute Analogs of calicheamicin gamma1I, method of making and using the same
US5269388A (en) 1991-11-12 1993-12-14 Stress-Tek, Inc. Weighing bed
GB9125768D0 (en) * 1991-12-04 1992-02-05 Hale Geoffrey Therapeutic method
ES2149768T3 (en) 1992-03-25 2000-11-16 Immunogen Inc CONJUGATES OF BINDING AGENTS OF CELLS DERIVED FROM CC-1065.
WO1994026087A2 (en) 1993-05-14 1994-11-24 Connor Kim C O Recombinant protein production and insect cell culture and process
CA2163345A1 (en) 1993-06-16 1994-12-22 Susan Adrienne Morgan Antibodies
US7119248B1 (en) 1994-04-12 2006-10-10 Miltenyi Biotec Gmbh Antibodies against epitopes with homology to self antigens, methods of preparation and applications thereof
KR100350260B1 (en) 1994-04-22 2003-01-06 교와 핫꼬 고교 가부시끼가이샤 Pyrroloindole derivatives
US5550246A (en) 1994-09-07 1996-08-27 The Scripps Research Institute Calicheamicin mimics
US5712374A (en) 1995-06-07 1998-01-27 American Cyanamid Company Method for the preparation of substantiallly monomeric calicheamicin derivative/carrier conjugates
US5714586A (en) 1995-06-07 1998-02-03 American Cyanamid Company Methods for the preparation of monomeric calicheamicin derivative/carrier conjugates
GB9603507D0 (en) 1996-02-20 1996-04-17 Isis Innovation Antibody variants
US7147851B1 (en) 1996-08-15 2006-12-12 Millennium Pharmaceuticals, Inc. Humanized immunoglobulin reactive with α4β7 integrin
GB2339430A (en) 1997-05-21 2000-01-26 Biovation Ltd Method for the production of non-immunogenic proteins
AU776910B2 (en) 1998-12-08 2004-09-23 Merck Patent Gesellschaft Mit Beschrankter Haftung Modifying protein immunogenicity
NZ517772A (en) 1999-11-24 2004-03-26 Immunogen Inc Cytotoxic agents comprising taxanes and their therapeutic use
DE60136527D1 (en) 2000-03-03 2008-12-24 Cambridge Antibody Tech ANTIBODIES TO EOTAXIN AND ITS USE
US6333410B1 (en) 2000-08-18 2001-12-25 Immunogen, Inc. Process for the preparation and purification of thiol-containing maytansinoids
US7465790B2 (en) 2000-10-09 2008-12-16 Isis Innovation, Inc. Therapeutic antibodies
US20020132983A1 (en) 2000-11-30 2002-09-19 Junghans Richard P. Antibodies as chimeric effector cell receptors against tumor antigens
CA2467633C (en) 2001-12-03 2012-03-27 Abgenix, Inc. Antibody categorization based on binding characteristics
AU2003217912A1 (en) * 2002-03-01 2003-09-16 Xencor Antibody optimization
AU2003291281A1 (en) 2002-11-01 2004-06-07 The Ohio State University Research Foundation Cytogenetic abnormalities that are predictive of response to therapy for chronic lymphocytic leukemia
CN1225480C (en) * 2002-12-18 2005-11-02 马菁 Anti CD52 monoclonal antibody, coding sequence and use thereof
US7534427B2 (en) 2002-12-31 2009-05-19 Immunomedics, Inc. Immunotherapy of B cell malignancies and autoimmune diseases using unconjugated antibodies and conjugated antibodies and antibody combinations and fusion proteins
KR20060002896A (en) * 2003-03-31 2006-01-09 기린 비루 가부시키가이샤 Method of inducing differentiation and proliferating regulatory t cell by anti-cd52 antibody and medicinal composition therefor
US7709224B2 (en) 2003-06-03 2010-05-04 Biosante Pharmaceuticals, Inc. Compositions and methods for enhanced expression of recombinant polypeptides from a single vector using a peptide cleavage site
US7264806B2 (en) * 2003-11-01 2007-09-04 Biovation Ltd. Modified anti-CD52 antibody
US20060204496A1 (en) * 2003-11-28 2006-09-14 Tetsuo Kojima Agonist antibody against heteroreceptor
ITRM20030601A1 (en) 2003-12-24 2005-06-25 Lay Line Genomics Spa METHOD FOR THE HUMANIZATION OF HUMANIZED ANTIBODIES AND ANTIBODIES WITH IT OBTAINED.
US7655229B2 (en) * 2004-09-02 2010-02-02 Chan Andrew C Anti-FC-gamma RIIB receptor antibody and uses therefor
ZA200701783B (en) * 2004-09-02 2009-10-28 Genentech Inc Anti-Fc-gamma RIIB receptor antibody and uses therefor
EP1850873B1 (en) 2005-02-08 2018-11-28 Genzyme Corporation Antibodies to tgfbeta
KR20080039843A (en) * 2005-05-24 2008-05-07 아베스타 겐그레인 테크놀로지스 피브이티 리미티드 Recombinant method for the production of a monoclonal antibody to cd52 for the treatment of chronic lymphocytic leukemia
PT2460831T (en) 2005-05-27 2017-01-17 Biogen Ma Inc Tweak binding antibodies
ES2382164T3 (en) * 2005-12-30 2012-06-05 Merck Patent Gmbh Anti-IL-6 antibodies that prevent the binding of IL-6 in complex with IL-6R () to GP130
EP2012814B1 (en) * 2006-04-12 2013-05-22 Genzyme Corporation Methods of treating autoimmune diseases
KR101583587B1 (en) 2006-09-13 2016-01-08 젠자임 코포레이션 -1 treatment of multiple sclerosis ms with campath-1h
US20100135998A1 (en) 2007-02-28 2010-06-03 Schering Corporation Combination therapy for treatment of immune disorders
US20100178293A1 (en) * 2007-06-22 2010-07-15 Olaf Weber Use of antibodies against the cd52 antigen for the treatment of neurological disorders, particularly transmissible spongiform encephalopathy and alzheimer's disease
TWI529247B (en) 2009-05-13 2016-04-11 建新公司 Anti-human cd52 immunoglobulins
EP3345620B1 (en) 2009-05-13 2024-08-28 Genzyme Corporation Methods and compositions for treating lupus
EP2429584A4 (en) 2009-05-13 2013-02-20 Genzyme Corp Methods and compositions for treatment
SG10201704269RA (en) 2009-07-15 2017-06-29 Aimm Therapeutics Bv Gram-positive bacteria specific binding compounds
WO2012009568A2 (en) 2010-07-16 2012-01-19 Adimab, Llc Antibody libraries
ITMI20110376A1 (en) 2011-03-10 2012-09-11 Wilic Sarl FLUID COOLED AIRBRUSHER
GB201109238D0 (en) 2011-06-01 2011-07-13 Antitope Ltd Antibodies
AR095199A1 (en) 2013-03-15 2015-09-30 Genzyme Corp ANTI-CD52 ANTIBODIES
AU2015330869B2 (en) 2014-10-09 2021-07-08 Genzyme Corporation Glycoengineered antibody drug conjugates
US20200299399A1 (en) 2017-04-21 2020-09-24 Genzyme Corporation Treatment of Multiple Sclerosis with Anti-CD52 Antibodies

Also Published As

Publication number Publication date
TW201043694A (en) 2010-12-16
KR101537840B1 (en) 2015-07-22
BRPI1013085A2 (en) 2020-11-03
HK1205152A1 (en) 2015-12-11
EP2998405A1 (en) 2016-03-23
TW201636367A (en) 2016-10-16
AU2010249003B2 (en) 2015-08-20
TWI614267B (en) 2018-02-11
JP2016093194A (en) 2016-05-26
MY160126A (en) 2017-02-28
US11945874B2 (en) 2024-04-02
RU2016142225A (en) 2018-12-18
EP3683317A3 (en) 2020-09-30
US20220010024A1 (en) 2022-01-13
HK1222682A1 (en) 2017-07-07
ZA201108077B (en) 2013-01-30
SG10201608169QA (en) 2016-11-29
CA2761800A1 (en) 2010-11-18
WO2010132659A3 (en) 2011-01-06
EP2429582A2 (en) 2012-03-21
NZ621170A (en) 2015-08-28
US20200040091A1 (en) 2020-02-06
KR20140102764A (en) 2014-08-22
CN110016081A (en) 2019-07-16
WO2010132659A2 (en) 2010-11-18
JP2012526558A (en) 2012-11-01
KR20120111932A (en) 2012-10-11
RU2603743C2 (en) 2016-11-27
JP5894912B2 (en) 2016-03-30
RU2011150516A (en) 2013-06-20
EP2998405B1 (en) 2019-12-11
US20140341910A1 (en) 2014-11-20
MX2011012047A (en) 2011-12-14
CA2761800C (en) 2016-09-27
AU2010249003A1 (en) 2011-11-03
AR076770A1 (en) 2011-07-06
EP3683317A2 (en) 2020-07-22
NZ596384A (en) 2014-03-28
TW201825115A (en) 2018-07-16
KR20160005143A (en) 2016-01-13
KR20170113704A (en) 2017-10-12
JP2014195474A (en) 2014-10-16
US20120100152A1 (en) 2012-04-26
CA2939492C (en) 2019-03-19
US8617554B2 (en) 2013-12-31
IL216141A0 (en) 2012-01-31
JP2018029624A (en) 2018-03-01
IL216141B (en) 2018-11-29
SG176060A1 (en) 2011-12-29
CN102459628A (en) 2012-05-16
IL262639A (en) 2018-12-31
US20160208010A1 (en) 2016-07-21
CN104231084A (en) 2014-12-24
EP2429582A4 (en) 2013-01-23
CA2939492A1 (en) 2010-11-18
KR20160103160A (en) 2016-08-31
CN104231084B (en) 2019-04-23

Similar Documents

Publication Publication Date Title
US11945874B2 (en) Anti-human CD52 immunoglobulins
AU2014233685B2 (en) Anti-CD52 antibodies
AU2017202364B2 (en) Anti-human CD52 immunoglobulins
AU2014200771B2 (en) Monoclonal antibodies
OA17634A (en) Anti-CD52 antibodies.

Legal Events

Date Code Title Description
MM4A Annulment or lapse of patent due to non-payment of fees